ABSTRACT
Organismal size depends on the interplay between genetic and environmental factors. Genome-wide association (GWA) analyses in humans have implied many genes in the control of height but suffer from the inability to control the environment. Genetic analyses in Drosophila have identified conserved signaling pathways controlling size; however, how these pathways control phenotypic diversity is unclear. We performed GWA of size traits using the Drosophila Genetic Reference Panel of inbred, sequenced lines. We find that the top associated variants differ between traits and sexes; do not map to canonical growth pathway genes, but can be linked to these by epistasis analysis; and are enriched for genes and putative enhancers. Performing GWA on well-studied developmental traits under controlled conditions expands our understanding of developmental processes underlying phenotypic diversity.
AUTHOR SUMMARY Genetic studies in Drosophila have elucidated conserved signaling pathways and environmental factors that together control organismal size. In humans, hundreds of genes are associated with height variation, but these associations have not been performed in a controlled environment. As a result we are still lacking an understanding of the mechanisms creating size variability within a species. Here, under carefully controlled environmental conditions, we identify naturally occurring genetic variants that are associated with size diversity in Drosophila. We identify a cluster of associations close to the kek1 locus, a well-characterized growth regulator, but otherwise find that most variants are located in or close to genes that do not belong to the conserved pathways but may interact with these in a biological network. Many of these genes have a conserved role in humans. We validate 33 novel growth regulatory genes that participate in diverse cellular processes, most notably cellular metabolism and cell polarity. This study is the first genome-wide association analysis of natural variants underlying size in Drosophila and our results complement the knowledge we have accumulated on this trait from mutational studies of single genes.
INTRODUCTION
How animals control and coordinate growth among tissues is a fundamental question in developmental biology. A detailed mechanistic but global understanding of the processes taking place during normal physiological development is furthermore relevant for understanding pathological growth in cancers. Classical genetic studies in Drosophila have revealed core molecular mechanisms governing growth control and have shed light on the role of humoral factors and the environment on adult size (1,2,3,4). Two major pathways regulate size, the Insulin/TOR pathway, which couples systemic growth to nutrient availability; and the Hippo tumor suppressor pathway, which controls cell survival and proliferation in developing organs (5,6,7). However, growth control is complex (8,9,10), and the interactions between components of these pathways with each other and with unknown molecules and extrinsic factors remain poorly understood. Studies focusing on single or a few genes can only capture individual aspects of the entire system of networks underlying this trait, which is especially problematic when individual alleles have subtle and context-dependent effects (11,12). Therefore, global genome-wide approaches are needed for a better understanding of the genetic control of size. One genome-wide approach is to study multifactorial natural genetic perturbations as they occur in a segregating, phenotypically diverse population.
Artificial selection experiments have revealed that naturally occurring populations of Drosophila melanogaster show abundant genetic variation for size, with heritabilities approaching 50% (13). Usually selection for size results in correlated responses in the same direction for all body parts and overall weight, indicating a common genetic architecture (14). Selection responses differ between populations but not between sexes (15). Body size is an important component of fitness in D. melanogaster since there are parallel clines in body size and correlated traits clines across different continents (17,18). Loci on chromosome 3R and 2R are, respectively, associated with body size and wing area (17, 18); interestingly, the majority of the 3R loci seem to be located within the polymorphic chromosomal inversion In(3R)Payne (19, 20). Candidate genes and variants associated with size within In(3R)Payne include hsr-omega, the microsatellite loci DMU25686 and AC008193, and genes in the Insulin signaling pathway (InR, Tsc1, Akt1) (21, 22). Similarly, the frequency of the polymorphic inversion In(2L)t is associated with a body size cline across several continents; genes in the IIS/TOR pathway (chico, Pten, Tor) are located in the inversion region and Pi3K21B and Idgfs 1-3 are located immediately proximal to it (22). Naturally segregating alleles in smp-30 (Dca) and InR have been causally associated with body weight (23, 24).
Recently, a long term selection experiment identified hundreds of loci with allele frequency differences between large and small populations (16), indicating that the genetic basis of naturally occurring variation in size is highly polygenic. Candidate loci were enriched for genes implicated in post-embryonic development, metamorphosis and cell morphogenesis. The genes included components of the EGFR, Hippo and many other growth pathways, as well as canonical IIS/TOR signaling genes. Therefore, dissecting the genetic basis of naturally occurring variation in body size has the potential to uncover novel variants in known loci affecting body size as well as identify novel genes.
The advent of next-generation sequencing technology has enabled the rapid and relatively cheap acquisition of complete genome sequences, and thereby the generation of very dense genotype information that enables genome-wide association (GWA) mapping with a much higher resolution than previously possible. GWA studies aim to link variation in quantitative traits to underlying genetic loci in populations of unrelated individuals genome-wide (25,26). GWAS have been pioneered (27,28) and widely applied in humans and are now a routinely used tool in model organisms such as Arabidopsis (29,30), Drosophila (31,32,33) and mouse (34) as well as in various crop (35,36) and domestic animal species (37,38,39,40,41), where they have substantially broadened our understanding of the genetics of complex traits. To date there are no GWA analyses of size in Drosophila, but GWA studies of height have revealed that many loci with small effect contribute to size variation in human populations (9,10,42,43), which contrasts with a much simpler genetic architecture of size in domestic animals, where as a consequence of breeding few loci have relatively large effect sizes that jointly explain a large proportion of size variation (38,44). Although many loci affecting human height have been identified by GWA analyses, deducing the underlying molecular mechanisms by which they affect size is challenging. Larger genome regions and not single genes are mapped; uncontrolled environmental variability makes it difficult to identify causal links between genotype and phenotype; and functional validation cannot be performed in humans (12,28,45,46,47).
In contrast to human studies, GWA studies in model organisms benefit from the feasibility of functional validation, more stringent environmental control and, when using inbred strains, the possibility of measuring many genetically identical individuals to obtain an accurate estimate of the phenotype for a given trait and genotype. All three factors can substantially improve the power of a GWA analysis. The establishment of the inbred, sequenced lines of the Drosophila Genetic Reference Panel (DGRP) (48,49) has made GWA analysis in Drosophila widely applicable. The DGRP lines harbor the substantial natural genetic variation present in the original wild population and show copious phenotypic variation for all traits assayed to date (31,32,33,48,50,51).
Here, we used the DGRP to perform single-and two-locus associations for size-related developmental traits in Drosophila. We find pervasive trait and sex-specificity of top variants, validate a substantial number of novel growth regulators, and extend our knowledge of the genetic control of size beyond existing growth regulatory networks.
RESULTS
Quantitative genetic analysis of size
We cultured 143 DGRP lines under conditions we had previously shown to reduce environmental influences on size (S1 Table, Fig. 1a) and measured five body and 21 wing traits (S1 Table, Fig. 1b). The cross trait genetic correlations were positive and generally high among all features except small veins and areas that were difficult to quantify accurately, indicating shared genetic architecture of the various size measures. We observed two modules of higher correlation, one formed by wing traits and the second by head/thorax traits (Fig. 1c, S1 Fig.), indicating that the genetic architecture is more similar among wing features and among head/thorax features than between traits of the wing and head/thorax. Principal component analysis (PCA) of 23 of the 26 size traits (L1, L6 and iarea8 were excluded since measuring these traits accurately was very difficult) revealed that the first two PCs explained nearly 75% of the observed phenotypic variation. The first component reflected an overall size element and the second component separated wing from head/thorax traits (Fig. 1d-f, S1 Fig.).
Given the observed redundancy of the phenotypes, we chose only one trait from each high-correlation module for further in-depth analysis: centroid size (CS, reflecting growth processes in the wing disc), and interocular distance (IOD, reflecting eye disc growth), respectively (Fig. 2a,b). IOD showed the lowest genetic correlation with CS of all head/thorax traits (0.46 in females and 0.51 in males). Interestingly, the allometric coefficient b describing the relationship CS = a*Xb (where X = IOD or TL) varied substantially between lines, from near independence (b=0) to hyperallometry (positive allometry b>1) (S2 Fig., S1 Table). We observed extensive phenotypic and genetic variation in both phenotypes (Fig. 2a, b, S1 and S2 Tables), which was reflected in the substantial broad-sense heritabilities . Furthermore, both traits showed significant genetic variation in sex dimorphism but similar heritability estimates for males and females and high cross-sex genetic (rMF) and phenotypic correlation (S1 Table). 15% of phenotypic variance in centroid size could be attributed to raising flies on different food batches, which only differed by the day on which they were prepared (according to the same protocol) (S1 Table). Though nutrition is a well-studied size-determining factor (52), we were surprised that even such small nutritional variation could have substantial phenotypic effects. Although the environmental effect of food batch was markedly lower for IOD (3%), we used batch-mean corrected phenotypes in all subsequent analyses to remove this effect.
Single-marker and gene based GWAS identify novel loci associated with size variation
To identify common loci contributing to size variation in Drosophila, we performed single marker GWA analyses (53) for 1,319,937 SNPs for a wing disc derived (CS) and an eye disc derived (IOD) size measure using Fast-LMM. This association method uses a linear mixed model to capture confounders such as population structure and cryptic relatedness. As the genetic correlation between CS and IOD was moderate (0.46 and 0.51 for females and males, respectively), we expected to map both shared and trait-specific SNPs. To find loci that specifically affect variation in wing size unrelated to the overall organismal size variation we constructed an additional phenotype (rCS) that had the effect of IOD on CS removed via regression. In addition to the effect of the food batch, two cosmopolitan inversions, In(2L)t and In(3R)Mo, were correlated with both CS and IOD and we addressed their effect on size by modeling their presence in the homozygous state (S2 Fig.), yielding the inversion-corrected phenotypes CSIC and IODIC. In(3R)P, which is known to be correlated with Drosophila size (19), was only homozygous in one line; therefore, we could not estimate its effect on size.
Only for one trait (IOD in females) did we observed significantly associated SNPs when applying a stringent Bonferroni corrected p-value threshold of 3.8×10-08. However, their significance dropped below the genome-wide level (pmin=3.94×10-06) when we applied GWAS on rank-normalized IOD, which is probably due to an outlier line (>4SD) in the minor allele class of these SNPs. Overall, the p-values between normalized and non-normalized GWAS showed good correlation (S3 Fig.).The six SNPs were all located in a cluster on chromosome 2L (2L: 12’805’398 – 12’806’812), 12-13kb upstream of the gene encoding the EGFR pathway regulator kek1 (Fig. 3a,c). Three more SNPs in this locus were annotated to kek1, but did not survive Bonferroni correction. All nine SNPs formed a haplotype, with lines having either all minor or all major alleles of these SNPs, and the minor allele haplotype was associated with an increased IOD (Figs. 3b,d, S3 Fig.). 198 SNPs are located in the region approximately 20kb upstream of kek1. This region showed high conservation between species (DGRP Freeze 2 genome browser, http://genome.ucsc.edu) and several blocks of higher LD are formed across it (Fig. 3b, S3 Fig.), which could be attributable to its proximity to In(2L)t (2L: 2’400’000 – 12’900’000). However, none of the lines with the minor allele haplotype was either homo-or heterozygous for this inversion, and they were distributed across all four food batches (S3 Fig.). Interestingly, a noncoding RNA, CR43818, is in the 20kb upstream region of kek1, and the region was spanned by the intron of CG9932, a poorly characterized gene that interacts genetically with Bx and Chi during wing development (54). Clearly there are signs for functionality of this locus, and several good candidates for causal variants. Further experiments are required to elucidate the molecular mechanism of this association and whether this may even be connected to In(2L)t.
As QQ-plots showed a departure from uniformity for p-values below 10-05 (S4 and S5 Figs.), and this threshold has been used for reporting associations in previous DGRP studies (48) we picked candidate loci using this nominal significance threshold for hypothesis generation and functional validation. The corresponding q-values for each SNP are listed in S3 Table. This yielded between 31 and 51 SNPs for females and between 17 and 36 SNPs for males, with little overlap between top associations and moderate correlation of overall SNP ranks between sexes (S3 and S4 Tables; S6, S7 and S8 Figs.), consistent with significant sex by line variances and departure of the cross-sex genetic correlations from unity in the quantitative genetic analyses.
Correcting for the segregation of polymorphic inversions generally enhanced the power of the GWA analyses, as is evident by more loci reaching nominal significance. Nevertheless, the majority (65-86%) of SNPs from the GWA analysis with uncorrected trait values remained candidates in the GWA analysis with corrected phenotypes. Somewhat surprisingly, despite the significant genetic correlation between CS and IOD, no candidate SNPs were shared between these phenotypes (Fig. 3e, S4 Table). In both sexes, approximately one-third of top SNPs was shared between the absolute and relative CS GWA analyses, suggesting variation in relative versus absolute organ size may be achieved through genetic variation at both shared and private loci.
Nominally associated variants predominantly mapped to intergenic regions, but were nevertheless enriched in gene regions (p<0.001, hypergeometric test) (Fig. 3f, S5 Table), demonstrating that associations were not randomly distributed across the genome. For gene-level analyses we determined candidates for each phenotype as genes having a nominally significant SNP in or within 1kb of their transcribed region, yielding a total of 107 genes over all phenotypes. Only the candidate gene sets for rCS were enriched for STRING curated interactions and only the candidate list for CSF was enriched for functional categories (positive regulation of Rho signal transduction and melanotic encapsulation of foreign target), though growth was among the top categories for CSMIC (FDR corrected p=0.08) (55). Given the large number of genes already known to play a role in growth control we were surprised that only few canonical growth genes contained or were close to nominally associated SNPs. Exceptions included several SNPs near or in the genes coding for Ilp8, TOR and EGFR pathway components and regulators of tissue polarity and patterning. However, some SNPs that narrowly missed the candidate reporting threshold localized to further growth regulatory genes, such as the Hippo pathway components ex and wts.
The small number of canonical growth pathway genes detected might be explained by the lack of SNPs with large effects in these genes, which is plausible considering the essential role of many growth regulators. We therefore wanted to test whether the combined signal of SNPs with small effects (each too small to reach significance on its own) across known growth genes might be significant. To this end we determined gene-based statistics using the sum of chi-squares VEGAS method (56), which computes a p-value for each gene considering all SNPs within a gene while correcting for gene length and linkage disequilibrium between SNPs. None of the genes reached genome-wide significance (p<3.75×10-06) (S6 Table). The overlap between the 20 top scoring genes from this analysis with our GWA candidate genes was small for each individual phenotype and even when combining the VEGAS analyses from all phenotypes only 11 of our 97 VEGAS top scoring genes contained a SNP that reached significance on its own in one of our GWA analyses. We did not find GO or interaction enrichment (55) and as in the individual GWA analyses, top candidates were largely novel with respect to growth control.
Functional validation of candidate genes reveals novel regulators of size
We selected a subset (41% to 69%) of candidates identified by each of our six wing size GWAS (CS, CSIC and rCS in both sexes) for functional validation by tissue-specific RNAi. A total of 64% to 79% of tested genes had significant effects on wing area (p<0.001, Wilcoxon rank sum test, S7 Table, Fig. 4a, S9 Fig.). We achieved similar validation rates for gene-based candidates. In contrast, only 42% of a set of 24 randomly selected genes had significant effects on wing size in females (S7 Table). The overall proportion of validated candidates versus random genes was significantly different (p=0.02, Fisher’s exact test) and Wilcoxon test p-values showed different distributions between candidate and random knockdowns (p=0.02, Wilcoxon test, S10 Fig.). This combined evidence suggests an advantage in power for identifying growth regulators by GWA over randomly testing genes. The validated candidates constitute 33 functionally diverse novel growth regulators (S11 Fig.).
Two-locus association reveals novel interactions
To place novel genes within the network of known growth pathways, we next performed tests for two-locus associations (57) to CSIC, IODIC and rCS in both sexes with SNPs in 306 growth genes as focal SNPs (S8 Table). This gene list was combined from genes listed as influencing wing development (The Interactive Fly, http://www.sdbonline.org/sites/fly/aimorph/wing.htm), commonly known growth genes from the IIS/TOR, EGFR and Hippo pathways, and growth regulators identified in screens by our group. This list is not comprehensive but should serve as a rough framework for the most relevant growth pathways. Overall, 15 interactions reached Bonferroni-corrected significance (p<7.9×10-13), but we observed none of our GWA candidates among the significant epistasis partners. Generally, more interactions reached genome wide significance in males than in females. The most significant interaction (CSMIC, p=5.79×10-15) occurred between mask, a positive regulator of JAK/STAT signaling (58) and tutl, a JAK/STAT target gene during optic lobe development (59) (Fig. 5). Furthermore, among the top five interactions we found one between nkd, a downstream target of Dpp (60), and the tyrosine phosphatase Ptp99A (CSFIC, p=8.79×10-14), which has been shown to interact with InR and the Ras signaling pathway (61,62). Furthermore, though we detected none of the significant interactions on DroID (63,64) mask and tutl, and PtP99A and nkd shared more DroID interactors than 95% of all possible pairs of the 32 genes involved in the significant interactions. Due to their already known growth-related functions we consider the interactions between these genes prime candidates for future functional validation.
To investigate whether our GWA candidates or genes from the ‘previously known’ catalog would be enriched further down the list, we lowered the stringency for reporting interactions to a discovery threshold of p<10-09. Counting only those interactions where the interacting SNP lay in or within 1kb of a gene (S8 Table, total 1,353 interactors across all phenotypes) we found enrichment for development, morphogenesis and signaling categories (Bonferroni corrected p<0.001) (55), which supports a role of these genes in growth control. Notably, the rCSM list (Fig. 5) was additionally enriched for genes involved in regulation of metabolic processes. Among them were 73 of the 306 genes in the ‘previously known’ catalog and 35 of our 107 overall GWAS candidates. However, these overlaps did not reach significance (p-value of 0.46 and 0.22, respectively). We next asked whether the candidate gene sets identified by normal GWAS and the epistasis approach were nevertheless biologically related to each other. To this end we used the STRING database (55), which revealed that the number of observed curated interactions between the two gene sets was much larger than expected by chance (p<<0.001). Analyzing pairwise interactions may thus help to place genes into pre-established networks.
Intergenic SNPs are preferentially located in regions with enhancer signatures and overlap lincRNA loci
Intergenic SNPs may be functional by changing the sequence of more distant regulatory elements or noncoding RNAs. We therefore tested whether intergenic GWAS candidate SNPs located to putative functional regions. We found enrichment (p<0.01, hypergeometric test) of SNPs lying in regions with H3K4Me1 or H3K27Ac, epigenetic signatures of active enhancers (S5 Table) (65), and in lincRNA loci (66), which have been implied in developmental regulation and are often enriched for trait-associated loci (67). Though only loci associated with IOD in females were enriched for SNPs localizing to lincRNA loci, we found one SNP lying in a lincRNA among the top variants for rCSF and IODFIC (S5 Table).
A SNP 2kb upstream (position 2L: 429144) of the Hippo pathway regulator ex narrowly missed the reporting threshold (p=1.7×10-05, CSM). However, its genomic location suggests this variant could affect a novel regulatory region for this gene. The region surrounding it was annotated with the enhancer methylation signatures H3K4Me1 and H3K27Ac and had assigned state 4 of the 9 state chromatin model suggestive of a strong enhancer (65,68). Further annotations included H3K9Ac, a mark of transcriptional start sites, histone deacetylase binding sites and an origin of replication. To further assess functionality, we investigated whether the sequence around this SNP was conserved across taxa by performing multiple sequence alignment using BLAST (69) (S9 Table). Indeed, the region immediately upstream of the D. melanogaster ex gene showed high similarity to ∼3kb regions slightly more upstream of expanded orthologs in the genomes of D. sechellia, D. yakuba and erecta (S9 Table, Fig. 4b). This combined evidence suggests a functional region immediately upstream of the D. melanogaster ex gene, but additional experiments are required to corroborate functionality and to establish an involvement in growth control and a mechanism for influencing size.
Human orthologs of candidate genes are associated with height, obesity and a variety of other traits
To investigate conservation to humans and further elucidate putative functions of candidate genes, we searched for orthologous proteins in humans. We found human orthologs (70) for 62 of our 107 GWA candidate genes, seven of which had a good confidence ortholog (score ≥ 3) associated with height, pubertal anthropometrics or growth defects (S10 Table). Furthermore, the GWAS candidates were enriched for human orthologs associated with height in a recent meta-analysis (p= 0.001) (10). The evidence for an involvement in growth control from GWAS in both organisms and experimental support from validation in Drosophila corroborates a biological function of these genes in the determination of body size.
DISCUSSION
We applied several GWA methods to developmental traits that have been extensively studied by single gene analyses in Drosophila as a complementary approach for identifying loci underlying size variation. Our single-marker GWAS revealed only one SNP cluster close to the known growth gene kek1 to be significantly associated with body size when using a conservative Bonferroni correction. Yet, in contrast to human GWA analyses, which require independent replication, we exploited the fact that our model organism is amenable to direct validation strategies and tested candidates corresponding to a much lower significance threshold of 10-05 for an involvement in size determination. Using tissue-specific RNAi, we validated 33 novel genes affecting Drosophila wing size. Nominally significant intergenic associations were preferentially located in regions with an enhancer signature and overlapped lincRNA loci. A SNP upstream of the expanded locus was in an evolutionarily conserved region, indicating the presence of a putatively functional element. A two-locus epistasis screen identified several genome-wide significant interactions between known growth genes and novel loci, showing that targeted epistasis analysis can be used to extend existing networks. Our study shows that despite limited statistical power, insights into the genetic basis of trait variation can be gained from analyzing nominal associations through functional and enrichment analyses and performing targeted locus-locus interaction studies.
Single-marker and two-locus GWA of size
Our study adds 33 novel growth genes and 15 genomic loci that may interact with known growth genes to the extensive number of loci already implied in size regulation from single gene studies. That only a few bona fide growth genes were among the nominally significant candidates could be due to selection against functional variation in natural populations and/or during subsequent inbreeding and/or that the effect sizes of SNPs in these genes are too small to be detected in the DGRP. Though it has been shown for other phenotypes that the identified loci seldom overlap between mutational and GWA approaches, we expected a higher overlap for size as this trait has been exceptionally intensively studied in Drosophila and as a result we have extensive prior knowledge on the underlying genes. Our validation of a substantial number of novel genes underscores the complementarity of the GWA approach to classical genetics and highlights the importance of probing natural variants. However, future studies would benefit from utilizing bigger population sizes in order to improve statistical power and from investigating populations with different geographic origins, to address population specificity of associated variants.
With the exception of the kek1 cluster, all the most significant wing size associations mapped to putative novel growth genes: CG6091, a de-ubiquitinating enzyme whose human ortholog has a role in innate immunity; CG34370, which was recently identified in a GWA analysis of lifespan and lifetime fecundity in Drosophila (71); and, surprisingly, dsx, a gene well characterized for its involvement in sex determination, fecundity and courtship behavior. dsx showed a significant effect on wing size in both sexes, CG6091 was only validated in males despite reaching a smaller p-value in the female GWAS, and CG34370 did not show a significant wing size change in either sex. Due to the obvious limitations of RNAi as a validation approach for SNPs we think it important to investigate the roles of CG6091 and CG34370 in growth control by other approaches before discarding them as false associations. As genes affecting growth also impact on general and reproductive fitness of organisms it is not surprising that most of the candidate variants in or close to genes lie in regulatory regions, potentially modulating splicing, RNA turnover or RNA/protein abundance. Our data support the general notion that intergenic SNPs can impact phenotypes, either by affecting transcript abundance of protein coding genes (e.g. through distal enhancer elements) or via noncoding RNAs, which have been shown to regulate many biological functions including cellular processes underlying growth (72,73,74).
There are few nonsense and missense SNPs among our candidates (one and six, respectively); these variants are prime contenders for effects on protein function. However, confirming such effects requires testing the SNP in an isogenic background. Knockdown of most candidate genes resulted in a small change in median wing size (-19.4% to 10.1%), indicating a redundant or mildly growth enhancing or suppressing role in this tissue, which may explain why they were not discovered by classical mutagenesis screens. However, larger effects might be observed upon ubiquitous knockout, knockdown or overexpression.
Epistasis analysis revealed 15 loci showing Bonferroni-significant interactions with SNPs in previously known growth genes, demonstrating the usefulness of this approach for extending existing biological networks. In addition to the interactions described in the main text, we note there is an interesting interaction between eIF2D (ligatin) and SNF4agamma (75). Furthermore, we found putative biological interactors for several GWA candidates among the top interactions that did not reach genome-wide significance e.g. Lar with InR. Lar can phosphorylate InR (61), so polymorphisms at these two loci could act synergistically to modulate InR activity. The enrichment of annotated interactions between our GWA candidates and epistasis partners shows that different analyses yielding different top associations uncover common underlying genetic networks. A similar combinatorial approach has been successful in study using the DGRP (33), underscoring that combinatorial approaches can help placing candidates from different analyses into a joint biological network, and provide a basis for further hypothesis driven investigation of the roles and connectivity of novel and known genes.
The kek1 locus
The region upstream of kek1 is the only locus where a larger genome region shows association. The minor allele frequency of this haplotype was between 4.7% and 6.2% (present in 7-10 lines). We explain the large effect of this locus by the fact that most lines with the minor alleles of the significant SNPs have an IOD that exceeds the 75th percentile of the IOD distribution in lines with the major allele. Obviously the effect may be overestimated due to relatively few lines having the minor allele, and due to effects of the genetic background. Nevertheless, the region contains some prime contenders for an effect on size: the SNPs lie in a region that could serve as a regulatory element for kek1 or the poorly characterized CG9932 that has been implied in wing disc development in another study (54). Furthermore, an uncharacterized noncoding RNA lies close by and could be linked to the SNP haplotype, due to generally higher LD in this region. Also, the region is spanned by In(2L)t, which itself shows association to size, and the observed effect could be due to this inversion. None of the lines with the minor allele haplotype had any copy of the inversion, which agrees with the observation that In(2L)t homozygous flies are relatively smaller than lines without the arrangement. On the other hand, only two lines in our dataset were homozygous for In(2L)t (DGRP_350 and DGRP_358), leaving many of the lines with the major allele with none or only one copy (nine lines) of the inversion, and we corrected for its presence, so we would not expect this to cause the association.
Biological roles of novel growth genes
Apart from expected processes like signaling, transcription, translation and morphogenesis, we validated genes involved in transmembrane transport, planar cell polarity (PCP), metabolism and immunity. A total of 24 single marker or two way interaction candidate genes from our GWA analyses were discovered to be enhancers or suppressors of major growth pathways in another study (76, S11 Table) and 15 were associated with nutritional variation in Drosophila (77), supporting their role in growth control. Importantly, the enrichment of GWA candidates for genes associated with human height not only supports their role in growth but also shows that results of GWA studies in Drosophila can be translated to orthologous traits and genes in humans. We do not see a large overlap between our candidates and the candidates identified by artificial selection on body size by Turner et al. (16), who identified many classical growth genes. We explain this discrepancy by the different methods to recover underlying genetic loci. Selection can enrich for rare alleles, while these cannot be probed in GWA. If these also had large effects, they would be strongly differentially selected for in the Turner study. In contrast, we would expect large effect alleles of canonical growth genes to be mostly rare in the DGRP lines, and thus not evaluated in the GWA. Furthermore, Turner et al. used a population from California, which likely has a different allele composition from our North Carolina population. A minor factor may be the rather coarse and general size measure used by Turner et al. Sieving selected for generally bigger flies, with no distinction between flies with bigger wings, heads, thoraxes, or legs that obstructed passage through the sieve. As growth of individual body parts is controlled by both systemic and organ intrinsic factors (1-4), and looking at overall size likely identifies the systemic, general factors, this could explain some of the discrepancy. We do not identify either InR or smp-30 (23,24). Both alleles have a relatively large effect. The smp-30 allele was identified in a population of different geographic origin and could thus not be present in the DGRP lines. The InR allele is an indel, and we only analyzed single nucleotide polymorphisms in this study. Although both genes likely contain further polymorphisms that are present in the DGRP, their effects may be far smaller and thus not detectable given the restricted size of the DGRP. In terms of chromosomal loci, we do identify SNPs on 3R, several of them located in the region spanned by In(3R)P (3R: 12,257,931 – 20,569,732). Also, we see a suggestion of In(3R)P correlating with size, but the inversion was present in too few lines of our dataset to reliably estimate its effect in a model.
Most of the loci we validated have not been previously linked with growth in Drosophila. The yeast ortholog of Mid1 (validated only in females but stronger association in males), is a stretch activated Ca2+ channel with a role in the polarized growth of mating projections (78,79). As mechanical tension plays a role during growth of imaginal discs, this channel could act in translating such signals to intracellular signaling pathways via the second messenger Ca2+. The human ortholog of another candidate, the transmembrane channel Trpm (associated and validated only in females), showed association with anthropometric traits during puberty, indicating a role during the postnatal growth phase. The mucin Muc68Ca, identified in the top 20 of the gene-based association to rCSF, showed one of the largest knockdown effects (14 and 15% reduction in size in females and males, respectively). Mucins form a protective layer around vital organs, and the expression pattern of Muc68Ca in the larval midgut concurs with a putative effect on growth via the control of intestinal integrity (80).
A dual role in PCP, the establishment of cell polarity within a plane in an epithelium, and growth control has been shown for many genes, which regulate these two processes via distinct but coordinated downstream cascades (81,82). Lar (no significant effect on size in validation), aPKC, the Fz target Kermit (83) and the motor proteins Dhc64C (not included in validation but contained a nonsense SNP reaching nominal significance) and Khc-73 (validated in males but stronger association in females, though with positive effect size), whose human ortholog is significantly associated with height, are implied in PCP establishment. Kermit and motor proteins act downstream in the PCP cascade and likely have specialized roles for this process, but PCP can itself impact on growth, as proper establishment of polarity provides the orientation of cell division, and loss of a PCP component in zebrafish causes a reduction in body length (84). Interestingly, kermit was a candidate interactor of EGFR, which acts in a combinatorial manner with Fz signaling in PCP (85), providing a biological basis for this interaction.
Metabolic genes are prime candidates for improving our understanding of growth, which depends on the amount of energy and precursors available for biosynthesis, and thus to metabolic coordination. The recent findings that the growth and PCP regulator Fat can couple growth and metabolism and mitochondrial proteins can causally affect growth pathway activity (86) underscore the importance of metabolic coordination. A missense SNP in the validated candidate Cep89, a gene involved in mitochondrial metabolism and growth in Drosophila and humans (87) was associated with most wing phenotypes. Elucidating the function of Cep89 and other validated candidates with putative roles in metabolism, e.g. CG3011, CG6084 and Fbp2, whose human ortholog has been linked to growth defects and cancer (e.g. 88), may provide further insight into this coordination.
Sexual dimorphism of size
Of the top 100 SNPs for each trait only 25% - 43% are shared between the sexes, a surprisingly small overlap given the high genetic and phenotypic correlations between sexes. In some cases the SNPs still lie in the same gene, implying that this gene differentially affects size in both sexes, but the responsible SNP is different. In other cases, we only detect associated SNPs for a gene in one sex. Here, the gene may affect size in both sexes but genetic variation in this gene affects size differentially in only one sex. As we have a low powered study this is only a hint and these results need to be further analyzed in a bigger population or by allele replacements using e.g. CRISPR/Cas9 to be corroborated. Unfortunately we cannot conclude anything about sex-specificity of our variants from the knockdown results. A knockdown is a very different perturbation from the effects of, for example, a regulatory variant. The knockdowns are performed in a different background than the one the association was discovered in, and they have much larger effect on the levels of a gene than a regulatory variant. So even though RNAi on a gene might show effects in males and females it does not exclude that different alleles of a SNP in this gene only affect wing size differentially in one sex.
Interestingly, an intronic SNP in the sex determination gene dsx had the lowest p-value in the female relative wing size GWAS but had a smaller effect size in males. Dsx is a transcription factor with sex-specific isoforms, and has many targets with sex- and tissue specific effects (89). We also observed sex-specificity for the genome-wide significant two-locus interactions. Considering that males use their wings to produce a courtship song that is instrumental for mating success, it may well be possible that selection pressure is different for male and female wing size or wing size in relation to other body parts. Indeed, the selection response for wing length seems to be more constrained in males (90). In our dataset, wing length is highly correlated with CS, our main wing size measure. Menezes et al. observed males with more elongated wings but also smaller males had the highest mating successes (91). These studies and our data suggest there may be subtle differences in the genetic networks underlying size determination in males and females in natural populations, a possibility that is neglected in single gene studies and thus would be worthwhile exploring.
Conclusions and future perspectives
Growth control has been well studied, particularly in Drosophila, where many genes and pathways affecting growth have been documented by mutational analyses. However, such screens are far from saturation and do not scale well to investigating effects of combinations of mutations. Here we took advantage of naturally occurring, multifactorial perturbations genome-wide to identify novel genes affecting growth and to place them in genetic interaction networks. Rather than deepening our understanding of growth control, the identification of ever more growth regulators raises new questions about how all these loci interact to govern growth. The challenge for the future will be to shift our focus from studying genes in isolation towards investigating them in the context of developmental networks, and to assess the effects of network perturbations on intermediate molecular phenotypes of transcript, protein and metabolite levels.
MATERIALS AND METHODS
Drosophila medium and strains
Fly food was prepared according to the following recipe: 100 g fresh yeast, 55 g cornmeal, 10 g wheat flour, 75 g sugar, 8 g bacto-agar and 1 liter tap water. Experiments were performed with 149 of the DGRP lines. RNAi lines used are listed in S7 Table.
Standardized culture conditions
Lines were set up in duplicate vials, with five males and five females per vial. After seven days, the parental flies were removed. From the F1, five males and five females were put together in duplicate vials and discarded after seven days of egg laying. From the F2, thirty males and thirty females were mated in a laying cage with an apple juice agar plate plus a yeast drop as food source and allowed to acclimatize for 24 hours. A fresh plate of apple juice agar plus yeast drop was then applied and flies were left to lay eggs for another 24 hours. From this plate, F3 L1 larvae were picked with forceps and distributed into three replicate vials, with 40 larvae per vial. The food surface in the vials was scratched and 100μl of ddH2O added prior to larvae transfer. The adult F3 flies were pooled from the three vials and frozen at -20°C approximately 1-2 days after eclosion. The whole experiment was performed in a dedicated incubator (DR-36VL, CLF Plant Climatics GmbH) with a 12-hour day-night cycle, constant humidity of 65 - 68% and constant temperature of 25.5°C +/- 1°C. Vials were shuffled every two days during the first and second round of mating but left at a fixed position in the incubator for the duration of the development of the F3 generation.
For the parental generation, lines were all set up on the same day on the same food batch. For the F1 matings, different food batches had to be used due to different developmental timing of the lines. F2 matings were set up using the same batch of apple agar plates and yeast for all lines. F3 larvae were distributed on four different food batches and the batch number was recorded for each line.
The control experiment (S1 Table) was performed using the same procedure as above, except that the same food batch was used for all flies of a generation. We used the DGRP lines DGRP_303, DGRP_732, DGRP_721 and DGRP_908 for this experiment because they had comparable generation times and set up ten replicates of each of these lines according to the standardized culture conditions.
Phenotyping and morphometric measurements
Depending on the number of flies available, between five and twenty-five flies per sex and line were measured for the dataset (median 25 flies per sex and line, mean 23 (CSfemales, CSmales, IODmales) and 24 for IODfemales; exact numbers are given in S2 Table). For the experimental generation we distributed a total of 19,200 larvae in four batches spaced throughout 1.5 weeks according to developmental timing, and the final dataset consisted of morphometric data of 6,978 flies, 3,500 females and 3,478 males. For the control experiment we phenotyped 25 flies per replicate, sex and line, resulting in a total of 2,000 flies (1,000 males, 1,000 females). Flies were positioned on a black apple agar plate and photographed using a VHX-1000 digital light microscope (KEYENCE). Morphometric body traits were measured manually using the VHX-1000 dedicated measurement software. If intact the right and otherwise the left wing was removed and mounted in water on a glass slide for wing image acquisition. Morphometric measurements were extracted from the wing images using WINGMACHINE (92) and MATLAB (MATLAB version R2010b Natick, Massachusetts: The MathWorks Inc.)
Centroid size was measured as the square root of the summed squared distances of 14 landmarks from the center of the wing (Fig. 1). Interocular distance was measured from eye edge to eye edge along the anterior edge of the posterior ocelli and parallel to the base of the head.
Quantitative genetic analysis
All analyses were performed in R Studio using the R statistical language version 2.15 (http://www.R-project.org). PCA was performed on data of individual flies using the package FactoMineR. Allometric coefficients (b) were determined for each line and sex from the model log(y) = log(a) + b * log(x), where y = CS and x = IOD or TL, using the lm() function in the stats package. 95% confidence intervals for the parameter b were computed using the confint() function in the stats package. The total phenotypic variance in the control experiment was partitioned using the mixed model Y = S + L + SxL + R(L) + ε, where S is the fixed effect of sex, L is the random effect of line (genotype), SxL is the random effect of line by sex interaction, R is the random effect of replicate and ε is the within line variance. The brackets represent that replicate is nested within line. The total phenotypic variance in the dataset was partitioned using the mixed model Y = S + L(F) + SxL(F) + F + ε, where S is the fixed effect of sex, L is the random effect of line (genotype), SxL is the random effect of line by sex interaction, F is the random effect of food batch and ε is the within line variance. The random effects of line and line by sex are nested within food batch, as each line was raised only on one of the four food batches. Models of this form were fitted using the lmer() function in the lme4 package in R. We also ran reduced models separately for males and females. The rand() function in the lmerTest package was used to assess significance of the random effects terms in the dataset.
Relative contributions of the variance components to total phenotypic variance was calculated as where represents any of , and stands for in the control dataset and for in the analysis of the GWAS dataset. = variance due to genotype, = variance due to genotype by sex interactions, = variance due to food, = variance due to replicate and = residual (intra-line) variance. The broad sense heritability for each trait was estimated as . The cross-sex genetic correlation was calculated as where is the variance among lines from the analysis pooled across sexes, σLF and, σLM are, respectively, the square roots of the among line variance from the reduced models of females and males. Similarly, cross-trait genetic correlations were calculated as where is the genetic covariance between traits A and B, and σGA and σGB are the square roots of the genetic variance for traits A and B, respectively. The phenotypic correlation between sexes was determined using the cor() function with method = “spearman” in R.
Phenotypes for GWAS
We found a large effect of food batch on CS, and inversions In(2L)t and In(3R)Mo were associated with IOD and to a lesser extent CS. We modeled these covariates using a mixed model. The food batch was modeled by a random effect and the rearrangements were coded as (0,1,2) depending on whether both, one or no inversion was present in the homozygous state. We did not observe correlation between Wolbachia infection status and any trait and thus did not include this as a covariate in the model. Specifically, the models used were: CSraw = α + X1β1 + X2β2 + Fu + ε, where X1 refers to the sex covariate, X2 refers to the inversion covariate, with n being the number of lines, with k being the number of food batches and Fu an (n,k)-indicator matrix, associating each line to its respective food batch. The GWA analyses were performed using the estimated residual of this model (CS = ε).
To find loci that specifically affected variation in wing size unrelated to the overall body size variation we constructed an additional phenotype (rCS) that had the effect of IOD on CS removed via regression: CSraw = α + IOD + X1β1 + Fu + ε, where X1 and Fu refer again to the sex-effect and the food batch effect. We did not model the inversions because the residuals of this model were not correlated with the inversions. The residuals ε from this regression were used as relative size phenotypes.
Association analyses
We performed GWA analyses using male and female line means. Genotypes for 143 of the 149 lines were obtained from the DGRP Freeze 2 website (http://dgrp2.gnets.ncsu.edu). Only SNPs that were missing in a maximum of ten lines and occurred in at least ten lines (7% of the measured lines, 1,319,937 SNPs in total) were used. GWA was performed using FaST-LMM (53) for separate sexes. This association method uses a linear mixed model to capture confounders such as population structure and cryptic relatedness. Association results were visualized using the manhattan() function in the R package qqman (93). To determine correlation between SNPs for a given phenotype we extracted the genotype of the top n SNPs (p<10-05) and calculated the correlation between genotypes at these loci across all DGRP lines used in the GWA analyses. We used the FaST-LMM SNP p-values to apply the sum of chi-squares VEGAS method (56) to calculate gene wise statistics. Gene boundaries were defined using annotation from popDrowser (http://popdrowser.uab.cat/gb2/gbrowse/dgrp/), but we included also SNPs lying within 1,000 bp up- or downstream of these margins. The correlation matrix was calculated from the genotypes themselves.
GO annotation and interaction enrichment
To determine enrichment of functional classes, annotate genes with functions and curated interactions among our candidate genes, we used the functional annotation and protein interaction enrichment tools from STRING (55).
RNAi validation
SNPs with an association p-value <10-05 lying in a gene region or ± 1 kb from a gene were mapped to that gene. From the gene based VEGAS analysis, we chose the top 20 genes from each list as candidates. RNAi lines for a subset of candidate genes for each wing phenotype were ordered from VDRC (94). For one gene, chinmo, there was no appropriate line available from VDRC and we instead tested two Bloomington lines (26777 (y[1] v[1]; P{y[+t7.7] v[+t1.8]=TRiP.JF02341}attP2) and 33638 (y[1] v[1]; P{y[+t7.7] v[+t1.8]=TRiP.HMS00036}attP2/TM3, Sb[1]), indicated in S7 Table with (BL)). For the random control knockdowns we tested a set of 24 genes that did not contain a significant SNP in or within 1 kb of their transcribed region. We did the random knockdowns only in females to more effectively assess more genes for the same labor. As we wanted to address the controls like an additional phenotype (random) we chose a number of genes comparable to the numbers of candidates for other phenotypes. We chose females because we generally had more candidate genes in females than in males. All RNAi lines used are listed in S7 Table. For wing size candidates, validation was performed by crossing males of the respective RNAi line to virgin females carrying the GAL4 transcriptional activator under the control of the nubbin (nub) promoter. The VDRC line containing a UAS-RNAi construct against the CG1315 (GD library, transformant ID 47097) gene served as a negative control for the knockdowns. We decided to use this line as reference because it was in the same background as most of our tester lines, an essential factor to consider when assessing genes that presumably only have a small effect on size upon knockdown. The CG1315 knockdown had never shown an effect in any setting and it allowed us to evaluate unspecific effects of RNAi knockdown on wing size. Prior to the experiment, driver lines were bred under controlled density to eliminate cross-generational effects of crowding on size. Wings were phenotyped as described above and wing area used as a phenotypic readout. Change in median wing area relative to the control was tested with a Wilcoxon rank sum test (function wilcoxon.test() in R) for each line and for separate sexes. If possible, 25 flies per cross and sex were phenotyped for statistical analysis, however sometimes the number of progeny was lower. The number of phenotyped flies per cross and sex is given in S7 Table. We used the fisher.test() function in R to determine if the proportion of validated genes was different among candidates and random lines, and the wilcoxon.test() function to test for a difference in median p-value between candidates and random lines. The comparison between candidate and random knockdowns was done for females exclusively as only this sex was measured for the random lines. Only genes not previously implied in wing development or growth control were included in the analysis, which excluded chinmo, aPKC, tws and Ilp8 from the candidates and EloA and spz5 from the random list.
Epistatic analyses
We explored epistatic interactions between SNPs lying within and 1 kb around genes that were previously found to be involved in growth or wing development in Drosophila against all DGRP SNPs with missingness <11 and present in at least 10% of the lines. We compiled a list of SNPs within and 1 kb up- or down-stream of genes that were previously known to play a role in growth control (14,137 SNPs) or wing development (43,498 SNPs) and used these as focal SNPs (S8 Table). All phenotypes were normalized to follow a standard normal distribution for this analysis to make sure that no severely non-normal distributions occurred within any of the four marker classes per locus. We used FasT-Epistasis (57) for calculating interactions for all pairs between the focal SNPs and the set of all SNPs satisfying the above criteria (1,100,811 SNPs). Bonferroni corrected significance would thus require p<7.9×10-13. Interactions were visualized using Circos (95). To calculate significance for the overlap between genes found via epistasis and a given gene list, we first positionally indexed all n SNPs that were used in the epistasis analysis. We recorded the set of indices of SNPs with p<10-09) yielding set K: K = {k: SNPk is an epistasis hit}. We then generated random samples. For random sample j, do:
For all elements in K, add a random integer rj between 0 and n-1. Define new index as the modulo n: , which yields . Given the shifted positions Kj, we look up the SNP positions PKj. For a given gene list, we record the number xj of gene regions that overlap a position in PKj. Let x be number of gene regions overlapping an epistasis hit. Our p-value estimate is then Papprox ≈ 1/m ∑1{xj ≥ x}.
Intergenic element enrichment analysis
We determined the number of SNPs from each GWA candidate list and the overall number of SNPs that located within modENCODE (65) elements annotated with Histone 3 lysine 4 monomethylation (H3K4Me1) or Histone 3 lysine 27 acetylation (H3K27Ac) or lincRNA loci. For the H3K4Me1/H3K27Ac enrichments we restricted ourselves to three developmental stages (L2, L3, pupae), which we considered to be the most relevant interval for gene activity affecting growth of imaginal discs. We obtained a table with lincRNAs in the Drosophila genome from the study of Young et al. (66) and searched for enrichment of SNPs located in those lincRNA loci. Enrichment was tested using a hypergeometric test (function phyper()) in R).
BLAST alignment
We downloaded the sequence of the region 10 kb upstream of the annotated transcription start site of the expanded locus (2L: 421227..431227) from FlyBase (96), as well as the sequence of the same relative region for seven of the twelve Drosophila species (97), which contained the ortholog of the expanded gene in the same orientation in the genome. We performed multiple sequence alignment using the discontiguous megablast option on NCBI BLAST (69).
Annotation with human orthologs
We combined candidate genes from GWA analyses of all phenotypes and searched for orthologs in humans using DIOPT-DIST (70). Enrichment of GWA candidates for genes with human orthologs associated with height (10) was determined with a hypergeometric test (function phyper() in R). We determined Drosophila orthologs of gene annotations of all associated SNPs (total 697), resulting in 374 ortholog pairs supported by at least 3 prediction tools, and searched for overlap of these orthologs with the 62 of our GWAS candidate genes that had a human ortholog supported by at least 3 prediction tools, which resulted in 12 matches. Of those, only five matches were supported by three or more prediction tools (score>=3) and we used only those for enrichment calculation. The total number of Drosophila-Human ortholog relationships (= 28,605) served as background (70).
AUTHOR CONTRIBUTIONS
EH, TM and SB conceived the approach. SV designed and performed experiments and SV and DL performed statistical analyses. SV wrote the manuscript and SV, DL, EH, SB and TM edited the manuscript.
SUPPORTING INFORMATION
S1 Table. Quantitative genetic analysis. Control experiment: Only 2% of total population variance in CS and IOD was due to flies coming from replicate vials, a negligible fraction compared to the 78% and 71% attributable to differences in genotype. This indicates that the standardized culture protocol sufficiently deals with confounding effects on size phenotypes. N=2000, 25 flies/sex of 10 replicates of four DGRP lines. Allometry: Allometric coefficients (b) calculated from the equation log(CS) = log(a) + b*log(trait) and their 95% confidence interval (CI) are given for the allometric relationships between CS and IOD and CS and TL for each line and sex. Though the CI varies substantially for some lines due to few data points used for fitting the models, the upper CI boundary is close to 0 for some (e.g. 28157 females (RAL228) for the CS-IOD relationship). QGA Dataset: Quantitative genetic analysis of CS and IOD in the dataset consisting of N=6978 flies from 149 DGRP lines. pSex = significance of fixed effect of sex, pLine = significance of random effect of Line, pSex x Line = significance of random effect of Line by sex interaction, pReplicate = significance of random effect of replicate, pFood = significance of random effect of foodbatch. Estimated parameters are variance due to genotype (VG), genotype by sex interaction (VGxS), food (VF), replicate (VR) and intra-line variance (VE), as well as the cross-sex genetic (rMF) and phenotypic correlation between sexes. H2 = broad-sense heritability and VP = total phenotypic variance. Phenotypic variation: Smallest and largest trait values and the percent difference are given per sex for each phenotype. Population means (Mean) and standard deviations (STD) are used to calculate the coefficient of variation (CV).
S2 Table. Phenotypic data. Raw data for all traits and line means (Mean), standard deviations (STD) and number of phenotyped flies (N) listed by sex for centroid size (CS) and interocular distance (IOD).
S3 Table. GWAS results. Nominally significant SNPs (p<10-05) from GWAS for Centroid size (CS), inversion modeled centroid size (CSIC), interocular distance (IOD), inversion modeled interocular distance (IODIC) and relative centroid size (rCS) in both sexes.
S4 Table. Between-sex and -phenotype overlap of nominally significant SNPs. GWAS SNPs: Number of nominally significant SNPs (p<10-05) identified in each of the GWAS and percent overlap between sexes. SNPs F = number of SNPs nominally significant in females, SNPs M = number of SNPs nominally significant in males, Common MF = number of SNPs nominally significant in both sexes, % M in F = percent nominally significant male SNPs also nominally significant in females, % F in M = percent nominally significant female SNPs also nominally significant in males. Between sex overlap: SNP and gene level overlap between sexes for different thresholds. Percent overlap of SNPs (exact associated positions), annotated SNPs (including annotation of SNPs located in intergenic regions where the annotation is often not reliable, as the next genes are frequently more than 20kb away), and genes (only includes SNPs that locate within or 1kb around a gene). A consistent difference in associated loci in terms of the exact SNP that is associated (top block) is detectable between sexes, though the loci apparently are located more or less in a similar region (middle block). For SNPs in or close to genes, the differences between sexes are more pronounced: of the top 100 associated genes about 50% overlap, while the other 50% are private to one sex but this percentage increases with inclusion of more genes (bottom block, top 10,000 is >90% overlap, in total there are around 14,000 genes in these lists). Between phenotype overlap: Proportion of nominally significant SNPs that are shared between phenotypes.
S5 Table. Enrichment analysis. Enrichment: Enrichment p-values for SNPs localizing to different genomic regions. LincRNA: LincRNA loci that overlap significant SNPs and their expression during different developmental stages. LincRNA data from Young et al. (54).
S6 Table. Top 20 genes for each trait identified by the VEGAS method. Last column indicates the percent change in median wing size of genes tested by RNAi, and asterisks (***) indicate significant change (p<0.001).
S7 Table. Validation results candidates and random genes. The lines showing a significant (p<0.001, Wilcoxon rank sum test) change in median wing area upon knockdown are shaded in grey. Crosses in columns pigmentation, bristles, veins indicate a slightly abnormal corresponding phenotype. N= number of individuals tested, Median = median wing area, Q25 and Q75 = first and third quartile of wing area distribution. MAF 3 or MAF 5 in brackets means a SNP in or near this gene was found among the top associated genes in a GWAS for wing size with a lower MAF cut-off (SNPs present in min. 3% or 5% of lines). This gene was tested for wing size since a SNP in it showed association to body size with the used MAF cutoff and thus a corresponding RNAi line was available. Overview: Overview validation results. Number of SNPs that were tested and the number and percentage that were validated for each trait. We tested the known genes chinmo, aPKC, tws and Ilp8 as positive controls, but did not include them in the calculation of these percentages. Fisher’s exact test: We performed a two-sided Fisher’s exact test to determine if the proportions of validated genes was different between candidates and random genes. The results are shown for different Wilcoxon test p-value validation thresholds. Only not previously known candidates and random lines were used (Ncandidates = 43, Nrandom = 22)
S8 Table. Epistasis results. Focal genes: Genes previously implied in growth regulation or wing development that were used as focal genes for epistasis. Top interactions (p<10-09) for female absolute inversion corrected wing size (CSFIC), male absolute inversion corrected wing size (CSMIC), female absolute inversion corrected body size (IODFIC), male absolute inversion corrected body size (IODMIC), female relative wing size (rCSF) and male relative wing size (rCSM). X is the interactor locus and Y the focal (= previously known) locus.
S9 Table. Multiple sequence alignment (MSA) results. Expanded orthologs: Genomic location of ex orthologs in 12 Drosophila species (82). Name of the ortholog, its genomic location and orientation are shown. For the MSA we only used species that contained the gene in the same orientation as D. melanogaster (grey). MSA details: Details of MSA of the 10kb region upstream of D. melanogaster ex gene. Sequence = genomic region in each species used in the MSA, Identity = percent identical nucleotides, Aligned Length = length of alignment, Query Cover = percent of the query sequence (D. melanogaster sequence) aligned to the sequence in the respective species, E-value = significance of alignment (expected number of high scoring pairs with score at least as high as the score of the current alignment), Score = strength of alignment.
S10 Table. Human orthologs of putative and validated Drosophila growth regulators and their association to human complex traits.
S11 Table. GWAS/epistasis candidates reported by other studies. Candidates found as suppressors or enhancers of major growth pathways by Schertel et al. (64). Candidates associated with nutritional indices in the study of Unckless et al. (65)
ACKNOWLEDGEMENTS
We thank Anna Troller, Benjamin Schlager and Anni Strässle for manual support during experiments. Stocks obtained from the Bloomington Drosophila Stock Center (NIH P40OD018537) and from the Vienna Drosophila RNAi Center were used in this study.
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