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Making scents of behavioural genetics: lessons from Drosophila

Published online by Cambridge University Press:  23 March 2011

ROBERT R. H. ANHOLT*
Affiliation:
Departments of Biology and Genetics and W. M. Keck Center for Behavioral Biology, North Carolina State University, Box 7617, Raleigh, NC 27695-7617, USA
*
*Corresponding author: Department of Biology, North Carolina State University, Box 7617, Raleigh, NC 27695-7617, USA. e-mail: [email protected]
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Summary

The expression of behaviours is influenced by many segregating genes. Behaviours are, therefore, complex traits. They have, however, unique characteristics that set them apart from physiological and morphological quantitative traits. First, behaviours are the ultimate expression of the nervous system. This means that understanding the genetic underpinnings of behaviours requires a neurobiological context, i.e. an understanding of the genes–brain–behaviour axis. In other words, how do ensembles of genes empower specific neural circuits to drive behaviours? Second, behaviours represent the interface between an organism and its environment. Thus, environmental effects are likely to make substantial contributions to determining behavioural outputs and genotype-by-environment interactions are expected to be prominent. It is important to differentiate between genes that contribute to the manifestation of the behavioural phenotype and genes that contribute to phenotypic variation in behaviour. The former are identified by classical mutagenesis experiments, whereas the latter can be detected through quantitative genetic approaches. Genes that contribute to phenotypic variation in behaviour harbour polymorphisms that provide the substrates for evolution. This review focuses on olfactory behaviour in Drosophila with the goal to illustrate how fundamental insights derived from studies on chemosensation can be applied to a wide range of behavioural phenotypes.

Type
Research Papers
Copyright
Copyright © Cambridge University Press 2011

1. Introduction: olfaction and Drosophila

Behaviours mediate adaptive responses that are essential for survival and reproduction. Thus, they represent the ultimate fitness traits and provide the mechanisms through which evolutionary forces can act. Most behaviours are dominated by sensory-motor processes in which sensory input is integrated, evaluated and acted on through motor output. Chemosensation is an important sensory input for most organisms and is essential for the localization of food, avoidance of toxins or predators and assessment of mating partners and oviposition sites. Chemical signals also drive other behaviours, including aggression, courtship and, in mammals, affiliative behaviours and parental care. Thus, studies on the genetics that underlies behavioural responses to chemical signals can provide biologically relevant information from which general principles can be derived which will be broadly applicable.

Drosophila melanogaster provides an excellent model system for studies on the genetic architecture of olfactory behaviour, since its olfactory system has been well characterized (Su et al., Reference Su, Menuz and Carlson2009) and flies are readily amenable to genetic, neuroanatomical, electrophysiological and behavioural manipulations. An important advantage of flies from a genetic perspective is the ability to generate a virtually unlimited number of individuals of the same genotype that can be grown under controlled environmental conditions. The ability to control both the genetic background and the environment precisely, together with the many publicly available genetic and genomic resources, makes Drosophila the perfect organism for studies aimed at dissecting the genetic underpinnings of behaviours.

2. Functional organization of the olfactory system of Drosophila

The main olfactory organs of Drosophila are the third antennal segments and the maxillary palps. The third antennal segment contains about 1200 olfactory receptor neurons housed in three morphologically distinct classes of sensilla: basiconic, coeloconic and trichoid sensilla. The maxillary palps contain about 120 olfactory sensory neurons in basiconic sensilla (Stocker, Reference Stocker1994; Shandbhag et al., Reference Shandbhag, Muller and Steinbrecht1999; Su et al., Reference Su, Menuz and Carlson2009). The sensilla are porous structures that contain two – or sometimes in the third antennal segment four – chemosensory neurons that express odorant receptors. They also contain supporting cells that secrete odorant-binding proteins in the perilymph that surrounds the chemosensory dendrites of the olfactory receptor neurons (Shandbhag et al., Reference Shandbhag, Hekmat-Scafe, Kim, Park, Carlson, Pikielny, Smith and Steinbrecht2001; Galindo & Smith, Reference Galindo and Smith2001; Hekmat-Scafe et al., Reference Hekmat-Scafe, Scafe, McKinney and Tanouye2002). Odorant-binding proteins are the first components of the olfactory system to encounter odorants and are thought to facilitate transport of odorants to their receptors. Recent evidence suggests that they also play a fundamental role in odorant discrimination (Matsuo et al., Reference Matsuo, Sugaya, Yasukawa, Aigaki and Fuyama2007; Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007, Reference Wang, Lyman, Mackay and Anholt2010).

The morphological classes of sensilla are functionally distinct. Basiconic sensilla are dedicated to general odorant discrimination and each olfactory sensory neuron within the basiconic sensilla expresses one or sometimes two unique odorant receptors from a repertoire of 62 Or genes (Clyne et al., Reference Clyne, Warr, Freeman, Lessing, Kim and Carlson1999; Gao & Chess, Reference Gao and Chess1999; Vosshall et al., Reference Vosshall, Amrein, Morozov, Rzhetsky and Axel1999). Each unique odorant receptor dimerizes with a common odorant receptor, the Or83b receptor (Larsson et al., Reference Larsson, Domingos, Jones, Chiappe, Amrein and Vosshall2004; Benton et al., Reference Benton, Sachse, Michnick and Vosshall2006), and activation of this complex by odorants results in the opening of a cation channel that depolarizes the olfactory sensory neuron (Sato et al., Reference Sato, Pellegrino, Nakagawa, Nakagawa, Vosshall and Touhara2008; Wicher et al., Reference Wicher, Schäfer, Bauernfeind, Stensmyr, Heller, Heinemann and Hansson2008). Coeloconic sensilla are enriched in a cavity of the third antennal segment, the sacculus, and express odorant receptors that resemble ionotropic glutamate receptors (Benton et al., Reference Benton, Vannice, Gomez-Diaz and Vosshall2009). The functions of this family of receptors, which is encoded by 61 functional Ir genes, are not clear, but they respond to odorants that include ammonia and phenyl acetaldehyde (Benton et al., Reference Benton, Vannice, Gomez-Diaz and Vosshall2009). Furthermore, in larvae of the mosquito Anopheles gambiae behavioural responses to butylamine are mediated via Ir receptors independent of classical Or receptors (Liu et al., Reference Liu, Pitts, Bohbot, Jones, Wang and Zwiebel2010). The T1 trichoid sensilla express the Or67d receptor and the Lush odorant-binding protein, which mediate recognition of the courtship pheromone 11-cis-vaccenyl acetate (Xu et al., Reference Xu, Atkinson, Jones and Smith2005; Ha & Smith, Reference Ha and Smith2006; Kurtovic et al., Reference Kurtovic, Widmer and Dickson2007). In addition, specialized sensilla in the third antennal segment express receptors that recognize carbon dioxide (Jones et al., Reference Jones, Cayirlioglu, Kadow and Vosshall2007; Kwon et al., Reference Kwon, Dahanukar, Weiss and Carlson2007). These receptors, Gr21a and Gr63a, belong to a multigene family of gustatory receptors (Scott et al., Reference Scott, Brady, Cravchik, Morozov, Rzhetsky, Zuker and Axel2001).

The axons of olfactory neurons project bilaterally to spherical structures of neuropil, glomeruli, in the antennal lobe (Vosshall et al., Reference Vosshall, Wong and Axel2000). For example, the CO2 sensing neurons in the third antennal segment project to glomerulus V (Suh et al., Reference Suh, Wong, Hergarden, Wang, Simon, Benzer, Axel and Anderson2004, Reference Suh, Ben-Tabou de Leon, Tanimoto, Fiala, Benzer and Anderson2007). The antennal lobes contain about 43 individually identifiable glomeruli (Laissue et al., Reference Laissue, Reiter, Hiesinger, Halter, Fischbach and Stocker1999). Elegant studies in which the expression of green fluorescent protein (GFP) is driven by Or promoters have resulted in a detailed projection map from peripheral sensory neurons that express distinct Or receptors to specific glomeruli in the antennal lobes (Vosshall et al., Reference Vosshall, Wong and Axel2000). Electrophysiological studies revealed a stereotypic organization of olfactory sensory neurons in the maxillary palps (de Bruyne et al., Reference de Bruyne, Clyne and Carlson1999) and antenna (de Bruyne et al., Reference de Bruyne, Foster and Carlson2001), in which pairs of neurons with defined molecular response profiles always occur together. Systematic ectopic expression studies in which Or genes were expressed in a mutant sensillum that lacks expression of its endogenous odorant receptor (Dobritsa et al., Reference Dobritsa, van der Goes van Naters, Warr, Steinbrecht and Carlson2003) have provided extensive documentation of the molecular response profiles of a large fraction of Or receptors in Drosophila (Hallem & Carlson, Reference Hallem and Carlson2006).

Combinatorial activation of odorant receptors by odorants generates a pattern of peripheral activity that is translated into a temporally and spatially dynamic activation pattern of glomeruli in the antennal lobes (Su et al., Reference Su, Menuz and Carlson2009). This glomerular activation map is processed by local interneurons and transmitted via projection neurons to the mushroom bodies and lateral horn of the protocerebrum in the brain (Wong et al., Reference Wong, Wang and Axel2002; Marin et al., Reference Marin, Jefferis, Komiyama, Zhu and Luo2002; Jefferis et al., Reference Jefferis, Potter, Chan, Marin, Rohlfing, Maurer and Luo2007; Masse et al., Reference Masse, Turner and Jefferis2009; Su et al., Reference Su, Menuz and Carlson2009), where olfactory information is interpreted and coupled to an appropriate motor output.

3. Plasticity of the expression of chemosensory genes

The intimate relationship between an organism and its chemical milieu requires adaptations of its chemosensory gene repertoire both over evolutionary time as habitats change and speciation occurs, and during the lifetime of the individual as it experiences changes in its physical and social environment. It is, therefore, perhaps not surprising that odorant binding protein (Obp) and odorant receptor (Or) gene families evolve rapidly (Gardiner et al., Reference Gardiner, Barker, Butlin, Jordan and Ritchie2008; Kopp et al., Reference Kopp, Barmina, Hamilton, Higgins, McIntyre and Jones2008; Sánchez-Gracia & Rozas, Reference Sánchez-Gracia and Rozas2008). Duplication of ancestral genes has resulted in the formation of clusters of Obp and Or genes throughout the genome. Examination of Or genes in 12 Drosophila species shows frequent gains and losses of genes as well as chromosomal rearrangements (Nozawa & Nei, Reference Nozawa and Nei2007; Sánchez-Gracia et al., Reference Sánchez-Gracia, Vieira and Rozas2009). Sequence analyses of members of the Obp56a–i and Obp99a–d clusters in a population of inbred wild-derived Drosophila lines showed different histories of recombination with different signatures of selection, including balancing selection for Obp99d, which showed an unusual degree of polymorphism in this population (Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007). Several studies have reported the maintenance of segregating Obp null alleles (Takahashi & Takano-Shimizu, Reference Takahashi and Takano-Shimizu2005; Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007). Such alleles can be tolerated if compensated for by functional redundancy within the Obp family. The best documented example of evolutionary adaptation of Obp genes comes from the host plant specialization of Drosophila sechellia. This species feeds and oviposits on fruit of Morinda citrifolia in its habitat on the Seychelles islands. The Morinda fruit is toxic and repellant to other Drosophila species and avoidance of this fruit appears due to hexanoic acid and octanoic acid, which are sensed by chemosensory neurons on the tarsi. A 4 bp insertion in the Obp57e gene in D. sechellia prevents expression of this Obp and results in loss of avoidance of hexanoic acid and octanoic acid, allowing D. sechellia to be attracted to the fruit of M. citrifolia (Matsuo et al., Reference Matsuo, Sugaya, Yasukawa, Aigaki and Fuyama2007; Dworkin & Jones, Reference Dworkin and Jones2009). Co-evolution of detoxification mechanisms might protect against toxicity of the Morinda fruit and further enable host plant specialization (Dworkin & Jones, Reference Dworkin and Jones2009). The chemosensory system of D. sechellia has undergone especially rapid evolution and host specialization has resulted in the accelerated loss of chemoreceptor genes (McBride, Reference McBride2007).

Gene duplication processes during the evolution of chemosensory genes can allow subfunctionalization or neofunctionalization of daughter genes. The Or22a and Or22b genes provide an example of a recent duplication (Aguadé, Reference Aguadé2009). These genes are located in tandem on the chromosome and expressed together in the same olfactory sensory neurons, the ab3A neurons. However, Or22a expression alone is sufficient to account for the molecular response properties of these neurons (Dobritsa et al., Reference Dobritsa, van der Goes van Naters, Warr, Steinbrecht and Carlson2003). Gene duplication may also have led to functional divergence among the family of odorant binding proteins and led to co-option of these proteins for functions other than mediating olfaction (Arya et al. Reference Arya, Weber, Wang, Magwire, Serrano Negron, Mackay and Anholt2010). This notion is supported by the observation that the expression of Obp genes is altered following mating, exposure to starvation stress (Harbison et al., Reference Harbison, Chang, Kamdar and Mackay2005), during the development of alcohol tolerance (Morozova et al., Reference Morozova, Anholt and Mackay2006), and as a correlated response to artificial selection for divergent levels of copulation latency (Mackay et al., Reference Mackay, Heinsohn, Lyman, Moehring, Morgan and Rollmann2005), aggression (Edwards et al., Reference Edwards, Rollmann, Morgan and Mackay2006) and sensitivity to alcohol (Morozova et al., Reference Morozova, Anholt and Mackay2007). Furthermore, members of the Obp gene family are expressed not only in chemosensory tissues but also in non-chemosensory tissues, such as the fat body (Fujii & Amrein, Reference Fujii and Amrein2002) and the male accessory gland (Ayroles et al., Reference Ayroles, Carbone, Stone, Jordan, Lyman, Magwire, Rollmann, Duncan, Lawrence, Anholt and Mackay2009), where they may serve roles as carriers for lipophilic compounds.

The chemosensory gene repertoire is plastic and expression levels of Obp and Or genes change dynamically as individual flies go through different developmental stages and experience different physical and social environments (Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009). Exposure to concentrated vapours of ethanol causes a rapid down-regulation of olfactory gene expression, including the common Or83b receptor (Morozova et al., Reference Morozova, Anholt and Mackay2006). Transcriptional profiling showed altered expression levels of several Obp genes in D. melanogaster females following mating (McGraw et al., Reference McGraw, Gibson, Clark and Wolfner2004). The expression of chemoreceptor genes, especially the Obp genes, is characterized by extensive sexual dimorphism (Figs 1 and 2; Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009). Males and females utilize the chemosensory gene repertoire differently, which reflects the strong influence of sex environment on gene expression and the different functional demands that are placed on chemosensation in each sex, such as mate recognition versus selection of oviposition sites. A striking example of sex-specific functional modulation of chemoreceptor expression is the observation that in the malaria-transmitting mosquito, Anopheles gambiae, expression of the AgOR1 odorant receptor, which is expressed specifically in female antennae, is dramatically down-regulated following a blood meal (Fox et al., Reference Fox, Pitts, Robertson, Carlson and Zwiebel2001).

Fig. 1. Phenotypic plasticity in the expression of chemoreceptor genes dependent on the physiological state. Relative expression levels of chemoreceptor genes assessed by hybridization of mRNA extracts to cDNA expression microarrays show differences in the expression of four gustatory receptor (Gr), 12 odorant receptor (Or) and 23 odorant-binding protein (Obp) genes between virgin and mated females (a). In contrast, only 17 Obp genes along with Pino, which encodes Pinocchio that resembles an odorant-binding protein (Rollmann et al., Reference Rollmann, Mackay and Anholt2005), show altered expression in mated compared to virgin males (b). Red bars indicate genes that show altered regulation in both sexes and arrowheads indicate antagonistic regulation between males and females (adapted from Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009).

Fig. 2. Phenotypic plasticity in the expression of chemoreceptor genes dependent on the developmental stage and sex. Relative expression levels of chemoreceptor genes assessed by hybridization of mRNA extracts to cDNA expression microarrays show differential gene expression between larval and adult life stages. Sexual dimorphism is prevalent among chemoreceptor genes and members of gene clusters are often regulated independently (adapted from Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009).

Specific members of the Obp and Or gene families change expression levels in larval stages (Fig. 2) and during senescence, following mating (Fig. 1a, b), and under conditions of solitary growth or exposure to groups of same sex or opposite sex individuals (Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009). Expression of members of the same gene cluster can be regulated independently and analysis of covariant expression levels of chemosensory genes across different conditions reveals 20 small modules of chemosensory genes that are regulated in a coordinated manner (Fig. 3; Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009). Combinations of transcription factors acting on cis-regulatory elements either promote or inhibit the expression of specific Or genes (Ray et al., Reference Ray, van der Goes van Naters and Carlson2008), and the POU domain transcription factors acj6 and pdm3 have been implicated in modulating expression of odorant receptors in subsets of olfactory neurons (Tichy et al., Reference Tichy, Ray and Carlson2008; Bai et al., Reference Bai and Carlson2009; Arya et al., Reference Arya, Weber, Wang, Magwire, Serrano Negron, Mackay and Anholt2010; Bai & Carlson, Reference Bai and Carlson2010). However, the molecular mechanisms that regulate altered expression of chemosensory genes in response to changes in the environment remain to be elucidated.

Fig. 3. Cluster analysis of chemoreceptor expression across multiple environmental conditions. The chemosensory gene repertoire clusters in 20 relatively small co-regulated transcriptional modules. Note that Obp76a, also known as Lush, and its receptor Or67d group together in module 4 (adapted from Zhou et al., Reference Zhou, Stone, Mackay and Anholt2009).

4. Mutagenesis and pleiotropy

Whereas chemoreceptors mediate odorant recognition and discrimination, transmission and interpretation of this chemosensory information and the ensuing behavioural response are influenced by many genes. Early studies on the genetics of olfaction utilized classical mutagenesis approaches and identified, among others, genes essential for neurotransmission, neurodevelopment and regulation of the expression of chemoreceptor genes.

One of the first olfactory mutants identified was smellblind, an allele of paralytic, which encodes the classical voltage-gated sodium channel (Lilly & Carlson, Reference Lilly and Carlson1990). Other genes essential for neurotransmission that impact on olfactory behaviour include a second voltage-gated sodium channel (NaCP60E; Kulkarni et al., Reference Kulkarni, Yamamoto, Robinson, Mackay and Anholt2002) and the synaptic PDZ domain protein scribble (Ganguly et al., Reference Ganguly, Mackay and Anholt2003). A quantitative trait locus (QTL) mapping study identified an allele of another PDZ domain protein, discs lost (Vanaso), as a quantitative trait gene for variation in olfactory behaviour in a mapping population derived from Oregon R and 2b strains (Fanara et al., Reference Fanara, Robinson, Rollmann, Anholt and Mackay2002). P-element insertional mutations in neurodevelopmental genes, such as Sema-5C (Rollmann et al., Reference Rollmann, Yamamoto, Goossens, Zwarts, Callaerts-Végh, Callaerts, Norga, Mackay and Anholt2007) and neuralized (Rollmann et al., Reference Rollmann, Edwards, Yamamoto, Zwarts, Callaerts, Norga, Mackay and Anholt2008), also affect olfactory behaviour. In addition, a POU-domain transcription factor, acj6, that regulates Or gene expression in subsets of chemosensory sensilla in the maxillary palps and antennae (Bai et al., Reference Bai, Goldman and Carlson2009; Bai & Carlson, Reference Bai and Carlson2010) was also initially identified from a mutant screen (Ayer & Carlson, Reference Ayer and Carlson1991).

Transcriptional profiling in mutant backgrounds identified large numbers of genes with altered transcriptional regulation (Anholt et al., Reference Anholt, Dilda, Chang, Fanara, Kulkarni, Ganguly, Rollmann, Kamdar and Mackay2003). These genes fall into multiple biological function gene ontology categories and are also candidate genes that may contribute to olfactory behaviour. P-element insertional mutagenesis screens consistently yielded 4–6% of lines with aberrant olfactory behaviour, reflecting a large mutational target and confirming that a large proportion of the genome contributes to olfactory behaviour (Anholt et al., Reference Anholt, Lyman and Mackay1996; Sambandan et al., Reference Sambandan, Yamamoto, Fanara, Mackay and Anholt2006). The extreme multigenic nature of behavioural traits is also evident from the hundreds of genes that undergo altered transcriptional regulation as a result of artificial selection, such as selection for low or high aggression (Edwards et al., Reference Edwards, Rollmann, Morgan and Mackay2006) and sensitivity or resistance to alcohol (Morozova et al., Reference Morozova, Anholt and Mackay2007). Thus, behavioural phenotypes are emergent properties of ensembles of pleiotropic genes.

5. Genetic networks

Mutagenesis studies are valuable for identifying genes that contribute to a behavioural phenotype and placing such genes in a mechanistic context. A complete understanding of the genetic underpinnings of behaviour, as for any complex trait, requires elucidating the coordinated action of networks of genes which qualitatively and quantitatively determine the expression of the phenotype. Genetic networks can be constructed by regressing phenotypic values of inbred wild-derived lines of D. melanogaster on transcript abundance levels across the genome and analysing covariance among the residuals of such regressions (Ayroles et al., Reference Ayroles, Carbone, Stone, Jordan, Lyman, Magwire, Rollmann, Duncan, Lawrence, Anholt and Mackay2009). This has been done for sleep (Harbison et al., Reference Harbison, Carbone, Ayroles, Stone, Lyman and Mackay2009) and alcohol sensitivity (Morozova et al., Reference Morozova, Ayroles, Jordan, Duncan, Carbone, Lyman, Stone, Govindaraju, Ellison, Mackay and Anholt2009). Alternatively, genetic interactions can be inferred directly by measuring additive or non-additive effects on the phenotype of mutant alleles as double heterozygotes. This analysis requires a collection of mutations in the same genetic background. A half-diallel crossing design then allows detection of enhancer or suppressor effects in each double heterozygote by evaluating the difference of observed phenotypic values from those predicted from the average heterozygous effects of each parent in combination with all other mutations (Fig. 4a; Griffing, Reference Griffing1956). Such an analysis has been performed for olfactory behaviour and revealed extensive epistatic interactions among P-element alleles with P-element insertions that affect the avoidance response to benzaldehyde (Fedorowicz et al., Reference Fedorowicz, Fry, Anholt and Mackay1998; Sambandan et al., Reference Sambandan, Yamamoto, Fanara, Mackay and Anholt2006). Extensive epistatic interactions appear to be a general hallmark, at least for behavioural traits. Similar epistatic networks have been identified for startle behaviour (Yamamoto et al., Reference Yamamoto, Zwarts, Norga, Callaerts, Mackay and Anholt2008) and climbing behaviour (van Swinderen & Greenspan, Reference van Swinderen and Greenspan2005).

Fig. 4. Identifying epistatic interactions among co-isogenic P-element insertion mutants. (a) Diagram of the half-diallel crossing principle. The three sets of the major homologous chromosomes of Drosophila are colour coded with red bars indicating P-element insertion sites. The small fourth chromosome is not depicted. Crosses between a set of homozygous co-isogenic P-element insertion lines (five are shown in this example) allow separation of dominance from non-additive enhancer/suppressor effects. (b) The analysis depicted in (a) can identify ensembles of genes that engage in dynamic epistatic interactions. On the left (green background) is an epistatic ensemble of transposon-tagged genes that affect olfactory behaviour (Sambandan et al., Reference Sambandan, Yamamoto, Fanara, Mackay and Anholt2006); on the right (orange background) is an epistatic ensemble of transposon-tagged genes that affect startle behaviour (Yamamoto et al., Reference Yamamoto, Zwarts, Norga, Callaerts, Mackay and Anholt2008). Overlap between the networks (yellow background) highlights genes that participate in both networks, illustrating pleiotropy.

The vast extent of epistasis among a small group of independently isolated P-element-insertion mutants is surprising and reveals an extensive network of enhancer and suppressor effects among genes that contribute to the same phenotype. These epistatic interactions for olfactory behaviour are dynamic and manifested differently at different odorant concentrations, even though the main effects of the mutations are stable (Sambandan et al., Reference Sambandan, Yamamoto, Fanara, Mackay and Anholt2006). Whereas one might expect epistatic effects to be minor compared to the main mutational effects, this is not always the case. For example, a P-element insertion at the smi21F locus affects expression of a protein named Pinocchio thought to function in odorant removal from the perilymph (Rollmann et al., Reference Rollmann, Mackay and Anholt2005). The effect of this P-element insertion on olfactory avoidance behaviour to benzaldehyde was small and detected only in females (Anholt et al., Reference Anholt, Lyman and Mackay1996). However, the smi21F P-element insertion showed extensive epistasis (Fedorowicz et al., Reference Fedorowicz, Fry, Anholt and Mackay1998). In a recent study, Canton-S chromosomes containing P-element insertions that affect startle behaviour along with their co-isogenic P-element-free controls were introduced in multiple inbred wild-derived genetic backgrounds. The magnitude of effects of these P-element insertional mutations on startle behaviour was attenuated by naturally occurring modifiers and there was a virtual linear relationship between the magnitude of the main mutational effects and the epistatic suppressor effects (Yamamoto et al., Reference Yamamoto, Anholt and Mackay2009). Thus, the dynamics of epistatic interactions can shift the balance of effects on the phenotype of genes within a network during an individual's lifetime, but, perhaps paradoxically, provides robustness to genetic networks over evolutionary time by buffering the effects of newly arising mutations.

The prevalence of both epistasis and pleiotropy implies that the same genes form part of multiple epistatic networks which give rise to different behavioural phenotypes (Fig. 4b). For example, P-element-insertions in neuralized (neur) affect olfactory behaviour, aggression and startle behaviour (Rollmann et al., Reference Rollmann, Edwards, Yamamoto, Zwarts, Callaerts, Norga, Mackay and Anholt2008). Epistasis analysis reveals a different context for neur in relation to other transposon-tagged genes that affect olfactory behaviour (Sambandan et al., Reference Sambandan, Yamamoto, Fanara, Mackay and Anholt2006) and startle behaviour (Yamamoto et al., Reference Yamamoto, Zwarts, Norga, Callaerts, Mackay and Anholt2008). Moreover, the consequences of the transposon insertion depend on its precise insertion site and orientation. For example, different P-element-insertion alleles for neur located only a few base pairs apart differentially affect olfactory behaviour and aggression, and these effects are accompanied by changes in the structure of the mushroom bodies (Rollmann et al., Reference Rollmann, Edwards, Yamamoto, Zwarts, Callaerts, Norga, Mackay and Anholt2008).

6. Linking genetic variation to phenotypic variation

Much information on the genetic basis of complex traits comes from associating DNA polymorphisms with phenotypic variation. Unlike the human genome that is characterized by large linkage disequilibrium (LD) blocks (Gabriel et al., Reference Gabriel, Schaffner, Nguyen, Moore, Roy, Blumenstiel, Higgins, DeFelice, Lochner, Faggart, Liu-Cordero, Rotimi, Adeyemo, Cooper, Ward, Lander, Daly and Altshuler2002), LD in Drosophila decays rapidly over a few hundred base pairs as a result of the short generation time and, consequently, a more extensive history of recombination. A disadvantage of this limited LD is that it precludes the use of tagging Single Nucleotide Polymorphisms (SNPs) and necessitates obtaining complete sequence information for association studies. An advantage is that once a polymorphism has been identified to be associated with phenotypic variation, this polymorphism is likely to be – or at least to be closely linked to – the causal variant.

Association studies in Drosophila have become possible with the generation of a population of 345 lines obtained by 20 generations of inbreeding of isofemale lines from a natural Raleigh, NC, population. Genetic variation within individual lines is minimal, while the collection of inbred wild-derived lines as a whole preserves the genetic diversity present in the original natural population. A subset of 192 of these lines with fully sequenced genomes represents a publicly available resource, the Drosophila Genetic Reference Panel (DGRP), which enables genome-wide association studies in Drosophila (Mackay et al., Reference Mackay, Richards and Gibbs2008).

Prior to the availability of whole genome sequences from the DGRP, sequencing individual candidate genes from among the 345 lines has enabled insights in the relationship between variants in the DNA sequence and variation in behavioural phenotypes. Sequencing the Obp99a–d group has identified SNPs in Obp99a, Obp99c and Obp99d that were associated with variation in olfactory responses to benzaldehyde (Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007). Whereas responses to benzaldehyde in isogenic laboratory strains are always strongly repellent (Anholt et al., Reference Anholt, Lyman and Mackay1996), phenotypic variation in responses to this odorant in the wild-derived lines is far broader spanning the range from complete attraction to complete repulsion (Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007). Such an extensive phenotypic variation is not unique to olfactory behaviour, but has been observed for virtually every trait studied in these lines and often exceeds the phenotypic extremes that can be obtained through artificial selection (Ayroles et al., Reference Ayroles, Carbone, Stone, Jordan, Lyman, Magwire, Rollmann, Duncan, Lawrence, Anholt and Mackay2009; Morozova et al., Reference Morozova, Ayroles, Jordan, Duncan, Carbone, Lyman, Stone, Govindaraju, Ellison, Mackay and Anholt2009). When associations between polymorphisms in the Obp99a–d cluster and responses to the odorant acetophenone were analysed, SNPs associated with variation in olfactory responses to this odorant were identified in Obp99a, Obp99b and Obp99d (Wang et al., Reference Wang, Lyman, Mackay and Anholt2010). These polymorphic markers, however, were distinct from those associated with variation in olfactory behaviour to benzaldehyde. This is of interest as these two odorants are structurally similar, differing only in a methyl group. These studies showed that odorant-binding proteins recognize odorants in a combinatorial manner, but different SNPs in Obp genes generate odorant-specific individual variation in chemosensory behaviour.

It is of interest to note that most of the SNPs associated with variation in olfactory behaviour in the Obp99a–d group were SNPs in non-coding regions or synonymous substitutions in the coding region. SNPs in non-coding regulatory regions may affect variation in expression. Synonymous SNPs in the coding region can affect mRNA structure, stability, processing and/or translation efficiency (Wang et al., Reference Wang, Lyman, Shabalina, Mackay and Anholt2007). An even more striking pattern of SNP associations has been found in the Catsup gene, which encodes a negative regulator of tyrosine hydroxylase, which is essential for the biosynthesis of dopamine. Here, distinct polymorphisms have been associated with startle-induced locomotion, longevity and sensory bristle phenotypes (Carbone et al., Reference Carbone, Jordan, Lyman, Harbison, Leips, Morgan, DeLuca, Awadalla and Mackay2006) as well as sleep (Harbison et al., Reference Harbison, Carbone, Ayroles, Stone, Lyman and Mackay2009). Thus, within pleiotropic genes different polymorphisms may be associated with phenotypic variation in different traits.

7. Behavioural genetics: lessons from Drosophila and future frontiers

Studies on the genetics of olfactory behaviour in Drosophila have yielded several fundamental insights. First, the genetic architecture of behaviour consists of epistatic networks of pleiotropic genes. These networks are plastic and dynamic and modulated by the sex, the social and physical environment and the developmental history of the organism. Second, embedded in these overlapping genetic networks are matrices of polymorphisms that provide the instrument for evolutionary change. A large proportion of these polymorphisms are synonymous or in regulatory regions. Rather than changing the structure of the encoded protein, they may affect expression levels, mRNA structure, stability, processing and/or translation efficiency. A third important insight from studies of whole genome transcriptional profiles of mutants that contain a single P-element that affects olfactory behaviour is the discovery that a single mutation or polymorphism can have widespread effects throughout the transcriptome (Anholt et al., Reference Anholt, Dilda, Chang, Fanara, Kulkarni, Ganguly, Rollmann, Kamdar and Mackay2003). This is an important caveat for the interpretation of associations of polymorphisms with disease susceptibility in human population studies. Similarly, the prevalence of epistasis and environment-dependent phenotypic plasticity are likely to apply not only to behavioural phenotypes in model organisms but also to human quantitative traits. Finally, although many genes are pleiotropic and contribute to multiple phenotypes, different alleles harbouring different polymorphisms appear to be associated with different traits.

Thus far, studies on the genetic architecture of behaviour have been mostly descriptive. A daunting challenge for the future will be to predict behavioural outcomes based on analyses of their genetic underpinnings, while taking into account epistatic interactions and environmental effects. A necessary component of this challenge is to link gene expression networks to distinct neuronal populations. Ideally, one would like to monitor the dynamics of whole genome transcriptional profiles in single neurons or small defined neuronal populations in behaving animals. The pursuit of this goal depends on new technological advances in the future.

I would like to thank Dr Trudy F. C. Mackay for valuable discussions and critical reading of the manuscript. Work in the author's laboratory is supported by grants from the National Institutes of Health (GM059469, 5RC1ES018255, GM045146, AA016560 and GM076083).

References

Aguadé, M. (2009). Nucleotide and copy-number polymorphism at the odorant receptor genes Or22a and Or22b in Drosophila melanogaster. Molecular Biology and Evolution 26, 6170.CrossRefGoogle ScholarPubMed
Anholt, R. R. H., Lyman, R. F. & Mackay, T. F. C. (1996). Effects of single P-element insertions on olfactory behavior in Drosophila melanogaster. Genetics 143, 293301.Google Scholar
Anholt, R. R. H., Dilda, C. L., Chang, S., Fanara, J. J., Kulkarni, N. H., Ganguly, I., Rollmann, S. M., Kamdar, K. P. & Mackay, T. F. C. (2003). The genetic architecture of odor-guided behavior in Drosophila: epistasis and the transcriptome. Nature Genetics 35, 180184.CrossRefGoogle ScholarPubMed
Arya, G. H., Weber, A. L., Wang, P., Magwire, M. M., Serrano Negron, Y. L., Mackay, T. F. C. & Anholt, R. R. H. (2010). Natural variation, functional pleiotropy and transcriptional contexts of odorant binding proteins in Drosophila melanogaster. Genetics September 24 E-print ahead of publication.Google Scholar
Ayer, R. K. Jr. & Carlson, J. (1991). acj6: a gene affecting olfactory physiology and behavior in Drosophila. Proceedings of the National Academy of Sciences of the USA 88, 54675471.CrossRefGoogle ScholarPubMed
Ayroles, J. F., Carbone, M. A., Stone, E. A., Jordan, K. W., Lyman, R. F., Magwire, M. M., Rollmann, S. M., Duncan, L. H., Lawrence, F., Anholt, R. R. H. & Mackay, T. F. C. (2009). Systems genetics of complex traits in Drosophila melanogaster. Nature Genetics 41, 299307.CrossRefGoogle ScholarPubMed
Bai, L. & Carlson, J. R. (2010). Distinct functions of acj6 splice forms in odor receptor gene choice. Journal of Neuroscience 30, 50285036.Google Scholar
Bai, L., Goldman, A. L. & Carlson, J. R. (2009). Positive and negative regulation of odor receptor gene choice in Drosophila by acj6. Journal of Neuroscience 29, 1294012947.CrossRefGoogle ScholarPubMed
Benton, R., Sachse, S., Michnick, S. W. & Vosshall, L. B. (2006). Atypical membrane topology and heteromeric function of Drosophila odorant receptors in vivo. PLoS Biology 4, e20.Google Scholar
Benton, R., Vannice, K. S., Gomez-Diaz, C. & Vosshall, L. B. (2009). Variant ionotropic glutamate receptors as chemosensory receptors in Drosophila. Cell 136, 149162.Google Scholar
Carbone, M. A., Jordan, K. W., Lyman, R. F., Harbison, S. T., Leips, J., Morgan, T. J., DeLuca, M., Awadalla, P. & Mackay, T. F. C. (2006). Phenotypic variation and natural selection at catsup, a pleiotropic quantitative trait gene in Drosophila. Current Biology 16, 912919.CrossRefGoogle ScholarPubMed
Clyne, P. J., Warr, C. G., Freeman, M. R., Lessing, D., Kim, J. & Carlson, J. R. (1999). A novel family of divergent seven-transmembrane proteins: candidate odorant receptors in Drosophila. Neuron 22, 327338.CrossRefGoogle ScholarPubMed
de Bruyne, M., Clyne, P. J. & Carlson, J. R. (1999). Odor coding in a model olfactory organ: the Drosophila maxillary palp. Journal of Neuroscience 19, 45204532.CrossRefGoogle Scholar
de Bruyne, M., Foster, K. & Carlson, J. R. (2001). Odor coding in the Drosophila antenna. Neuron 30, 537552.Google Scholar
Dobritsa, A. A., van der Goes van Naters, W., Warr, C. G., Steinbrecht, R. A. & Carlson, J. R. (2003). Integrating the molecular and cellular basis of odor coding in the Drosophila antenna. Neuron 37, 827841.Google Scholar
Dworkin, I. & Jones, C. D. (2009). Genetic changes accompanying the evolution of host specialization in Drosophila sechellia. Genetics 181, 721736.CrossRefGoogle ScholarPubMed
Edwards, A. C., Rollmann, S. M., Morgan, T. J. & Mackay, T. F. C. (2006). Quantitative genomics of aggressive behavior in Drosophila melanogaster. PLoS Genetics 2, e154.CrossRefGoogle ScholarPubMed
Fanara, J. J., Robinson, K. O., Rollmann, S. M., Anholt, R. R. H. & Mackay, T. F. C. (2002). Vanaso is a candidate quantitative trait gene for olfactory behavior in Drosophila melanogaster. Genetics 162, 13211328.CrossRefGoogle Scholar
Fedorowicz, G. M., Fry, J. D., Anholt, R. R. H. & Mackay, T. F. C. (1998). Epistatic interactions between smell-impaired loci in Drosophila melanogaster. Genetics 148, 18851891.CrossRefGoogle ScholarPubMed
Fox, A. N., Pitts, R. J., Robertson, H. M., Carlson, J. R. & Zwiebel, L. J. (2001). Candidate odorant receptors from the malaria vector mosquito Anopheles gambiae and evidence of down-regulation in response to blood feeding. Proceedings of the National Academy of Sciences of the USA 98, 1469314697.CrossRefGoogle ScholarPubMed
Fujii, S. & Amrein, H. (2002). Genes expressed in the Drosophila head reveal a role for fat cells in sex-specific physiology. EMBO Journal 21, 53535363.CrossRefGoogle ScholarPubMed
Gabriel, S. B., Schaffner, S. F., Nguyen, H., Moore, J. M., Roy, J., Blumenstiel, B., Higgins, J., DeFelice, M., Lochner, A., Faggart, M., Liu-Cordero, S. N., Rotimi, C., Adeyemo, A., Cooper, R., Ward, R., Lander, E. S., Daly, M. J. & Altshuler, D. (2002). The structure of haplotype blocks in the human genome. Science 296, 22252229.CrossRefGoogle ScholarPubMed
Galindo, K. & Smith, D. P. (2001). A large family of divergent Drosophila odorant-binding proteins expressed in gustatory and olfactory sensilla. Genetics 159, 10591072.CrossRefGoogle ScholarPubMed
Ganguly, I., Mackay, T. F. C. & Anholt, R. R. H. (2003). scribble is essential for olfactory behavior in Drosophila. Genetics 164, 14471457.Google Scholar
Gao, Q. & Chess, A. (1999). Identification of candidate Drosophila olfactory receptors from genomic DNA sequence. Genomics 60, 3139.Google Scholar
Gardiner, A., Barker, D., Butlin, R. K., Jordan, W. C. & Ritchie, M. G. (2008). Drosophila chemoreceptor gene evolution: selection, specialization and genome size. Molecular Ecology 17, 16481657.CrossRefGoogle ScholarPubMed
Griffing, B. (1956). Concept of general and specific combining ability in relation to diallel crossing systems. Australian Journal of Biological Sciences 9, 463493.CrossRefGoogle Scholar
Ha, T. S. & Smith, D. P. (2006). A pheromone receptor mediates 11-cis-vaccenyl acetate-induced responses in Drosophila. Journal of Neuroscience 26, 87278733.CrossRefGoogle ScholarPubMed
Hallem, E. A. & Carlson, J. R. (2006). Coding of odors by a receptor repertoire. Cell 125, 143160.CrossRefGoogle ScholarPubMed
Harbison, S. T., Chang, S., Kamdar, K. P., Mackay, T. F. (2005). Quantitative genomics of starvation stress resistance in Drosophila. Genome Biology 6, R36.Google Scholar
Harbison, S. T., Carbone, M. A., Ayroles, J. F., Stone, E. A., Lyman, R. F. & Mackay, T. F. C. (2009). Co-regulated transcriptional networks contribute to natural genetic variation in Drosophila sleep. Nature Genetics 41, 371375.CrossRefGoogle ScholarPubMed
Hekmat-Scafe, D. S., Scafe, C. R., McKinney, A. J. & Tanouye, M. A. (2002). Genome-wide analysis of the odorant-binding protein gene family in Drosophila melanogaster. Genome Research 12, 13571369.Google Scholar
Jefferis, G. S., Potter, C. J., Chan, A. M., Marin, E. C., Rohlfing, T., Maurer, C. R. Jr. & Luo, L. (2007). Comprehensive maps of Drosophila higher olfactory centers: spatially segregated fruit and pheromone representation. Cell 128, 11871203.CrossRefGoogle ScholarPubMed
Jones, W. D., Cayirlioglu, P., Kadow, I. G. & Vosshall, L. B. (2007). Two chemosensory receptors together mediate carbon dioxide detection in Drosophila. Nature 445, 8690.Google Scholar
Kopp, A., Barmina, O., Hamilton, A. M., Higgins, L., McIntyre, L. M. & Jones, C. D. (2008). Evolution of gene expression in the Drosophila olfactory system. Molecular Biology and Evolution 25, 10811092.CrossRefGoogle ScholarPubMed
Kulkarni, N. H., Yamamoto, A., Robinson, K. O., Mackay, T. F. C. & Anholt, R. R. H. (2002). The DSC1 channel, encoded by the smi60E locus, contributes to odor-guided behavior in Drosophila melanogaster. Genetics 161, 15071516.Google Scholar
Kurtovic, A., Widmer, A. & Dickson, B. J. (2007). A single class of olfactory neurons mediates behavioural responses to a Drosophila sex pheromone. Nature 446, 542546.Google Scholar
Kwon, J. Y., Dahanukar, A., Weiss, L. A. & Carlson, J. R. (2007). The molecular basis of CO2 reception in Drosophila. Proceedings of the National Academy of Sciences of the USA 104, 35743578.Google Scholar
Laissue, P. P., Reiter, C., Hiesinger, P. R., Halter, S., Fischbach, K. F. & Stocker, R. F. (1999). Three-dimensional reconstruction of the antennal lobe in Drosophila melanogaster. Journal of Comparative Neurology 405, 543552.Google Scholar
Larsson, M. C., Domingos, A. I., Jones, W. D., Chiappe, M. E., Amrein, H. & Vosshall, L. B. (2004). Or83b encodes a broadly expressed odorant receptor essential for Drosophila olfaction. Neuron 43, 703714.CrossRefGoogle ScholarPubMed
Lilly, M. & Carlson, J. (1990). smellblind: a gene required for Drosophila olfaction. Genetics 124, 293302.CrossRefGoogle ScholarPubMed
Liu, C., Pitts, R. J., Bohbot, J. D., Jones, P. L., Wang, G. & Zwiebel, L. J. (2010). Distinct olfactory signaling mechanisms in the malaria vector mosquito Anopheles gambiae. PLoS Biology 8, e1000467.CrossRefGoogle ScholarPubMed
Mackay, T. F. C., Heinsohn, S. L., Lyman, R. F., Moehring, A. J., Morgan, T. J. & Rollmann, S. M. (2005). Genetics and genomics of Drosophila mating behavior. Proceedings of the National Academy of Sciences of the USA 102 (Suppl 1), 66226629.CrossRefGoogle ScholarPubMed
Mackay, T., Richards, S. & Gibbs, R. (2008). Proposal to sequence a Drosophila genetic reference panel: a community resource for the study of genotypic and phenotypic variation [white paper]. Available from http://flybase.org/Google Scholar
Marin, E. C., Jefferis, G. S., Komiyama, T., Zhu, H. & Luo, L. (2002). Representation of the glomerular olfactory map in the Drosophila brain. Cell 109, 243255.CrossRefGoogle ScholarPubMed
Masse, N. Y., Turner, G. C. & Jefferis, G. S. (2009). Olfactory information processing in Drosophila. Current Biology 19, R700R713.CrossRefGoogle ScholarPubMed
Matsuo, T., Sugaya, S., Yasukawa, J., Aigaki, T. & Fuyama, Y. (2007). Odorant-binding proteins OBP57d and OBP57e affect taste perception and host-plant preference in Drosophila sechellia. PLoS Biology 5, e118.CrossRefGoogle ScholarPubMed
McBride, C. S. (2007). Rapid evolution of smell and taste receptor genes during host specialization in Drosophila sechellia. Proceedings of the National Academy of Sciences of the USA 104, 49965001.Google Scholar
McGraw, L. A., Gibson, G., Clark, A. G. & Wolfner, M. F. (2004). Genes regulated by mating, sperm, or seminal proteins in mated female Drosophila melanogaster. Current Biology 14, 15091514.Google Scholar
Morozova, T. V., Anholt, R. R. H. & Mackay, T. F. C. (2006). Transcriptional response to alcohol exposure in Drosophila melanogaster. Genome Biology 7, R95.CrossRefGoogle ScholarPubMed
Morozova, T. V., Anholt, R. R. H. & Mackay, T. F. C. (2007). Phenotypic and transcriptional response to selection for alcohol sensitivity in Drosophila melanogaster. Genome Biology 8, R231.CrossRefGoogle ScholarPubMed
Morozova, T. V., Ayroles, J. F., Jordan, K. W., Duncan, L. H., Carbone, M. A., Lyman, R. F., Stone, E. A., Govindaraju, D. R., Ellison, C. R., Mackay, T. F. C. & Anholt, R. R. H. (2009). Alcohol sensitivity in Drosophila: translational potential of systems genetics. Genetics 83, 733745.Google Scholar
Nozawa, M. & Nei, M. (2007). Evolutionary dynamics of olfactory receptor genes in Drosophila species. Proceedings of the National Academy of Sciences of the USA 104, 71227127.CrossRefGoogle ScholarPubMed
Ray, A., van der Goes van Naters, W. & Carlson, J. R. (2008). A regulatory code for neuron-specific odor receptor expression. PLoS Biology 6, e125.Google Scholar
Rollmann, S. M., Mackay, T. F. C. & Anholt, R. R. H. (2005). Pinocchio, a novel protein expressed in the antenna, contributes to olfactory behavior in Drosophila melanogaster. Journal of Neurobiology 63, 146158.Google Scholar
Rollmann, S. M., Yamamoto, A., Goossens, T., Zwarts, L., Callaerts-Végh, Z., Callaerts, P., Norga, K., Mackay, T. F. C. & Anholt, R. R. H. (2007). The early developmental gene Semaphorin 5c contributes to olfactory behavior in adult Drosophila. Genetics 176, 947956.CrossRefGoogle ScholarPubMed
Rollmann, S. M., Edwards, A. C., Yamamoto, A., Zwarts, L., Callaerts, P., Norga, K., Mackay, T. F. C. & Anholt, R. R. H. (2008). Pleiotropic effects of Drosophila neuralized on complex behaviors and brain structure. Genetics 179, 13271336.Google Scholar
Sambandan, D., Yamamoto, A., Fanara, J. J., Mackay, T. F. C. & Anholt, R. R. H. (2006). Dynamic genetic interactions determine odor-guided behavior in Drosophila melanogaster. Genetics 174, 13491363.Google Scholar
Sánchez-Gracia, A. & Rozas, J. (2008). Divergent evolution and molecular adaptation in the Drosophila odorant-binding protein family: inferences from sequence variation at the OS-E and OS-F genes. BMC Evolutionary Biology 8, 323.CrossRefGoogle Scholar
Sánchez-Gracia, A., Vieira, F. G. & Rozas, J. (2009). Molecular evolution of the major chemosensory gene families in insects. Heredity 103, 208216.CrossRefGoogle ScholarPubMed
Sato, K., Pellegrino, M., Nakagawa, T., Nakagawa, T., Vosshall, L. B. & Touhara, K. (2008). Insect olfactory receptors are heteromeric ligand-gated ion channels. Nature 452, 10021006.Google Scholar
Scott, K., Brady, R. Jr., Cravchik, A., Morozov, P., Rzhetsky, A., Zuker, C. & Axel, R. (2001). A chemosensory gene family encoding candidate gustatory and olfactory receptors in Drosophila. Cell 104, 661673.Google Scholar
Shandbhag, S., Muller, B. & Steinbrecht, A. (1999). Atlas of olfactory organs of Drosophila melanogaster. 1. Types, external organization, innervations and distribution of olfactory sensilla. International Journal of Insect Morphology and Embryology 28, 377397.Google Scholar
Shandbhag, S. R., Hekmat-Scafe, D., Kim, M. S., Park, S. K., Carlson, J. R., Pikielny, C., Smith, D. P. & Steinbrecht, R. A. (2001). Expression mosaic of odorant-binding proteins in Drosophila olfactory organs. Microscopy Research Techniques 55, 297306.Google Scholar
Stocker, R. F. (1994). The organization of the chemosensory system in Drosophila melanogaster: a review. Cell and Tissue Research 275, 3–26.Google Scholar
Su, C. Y., Menuz, K. & Carlson, J. R. (2009). Olfactory perception: receptors, cells, and circuits. Cell 139, 4559.Google Scholar
Suh, G. S., Wong, A. M., Hergarden, A. C., Wang, J. W., Simon, A. F., Benzer, S., Axel, R. & Anderson, D. J. (2004). A single population of olfactory sensory neurons mediates an innate avoidance behaviour in Drosophila. Nature 431, 854859.Google Scholar
Suh, G. S., Ben-Tabou de Leon, S., Tanimoto, H., Fiala, A., Benzer, S. & Anderson, D. J. (2007). Light activation of an innate olfactory avoidance response in Drosophila. Current Biology 17, 905908.Google Scholar
Takahashi, A. & Takano-Shimizu, T. (2005). A high-frequency null mutant of an odorant-binding protein gene, Obp57e, in Drosophila melanogaster. Genetics 170, 709718.Google Scholar
Tichy, A. L., Ray, A. & Carlson, J. R. (2008). A new Drosophila POU gene, pdm3, acts in odor receptor expression and axon targeting of olfactory neurons. Journal of Neuroscience 28, 71217129.CrossRefGoogle ScholarPubMed
van Swinderen, B. & Greenspan, R. J. (2005). Flexibility in a gene network affecting a simple behavior in Drosophila melanogaster. Genetics 169, 21512163.Google Scholar
Vosshall, L. B., Amrein, H., Morozov, P. S., Rzhetsky, A. & Axel, R. (1999). A spatial map of olfactory receptor expression in the Drosophila antenna. Cell 96, 725736.CrossRefGoogle ScholarPubMed
Vosshall, L. B., Wong, A. M. & Axel, R. (2000). An olfactory sensory map in the fly brain. Cell 102, 147159.Google Scholar
Wang, P., Lyman, R. F., Shabalina, S., Mackay, T. F. C. & Anholt, R. R. H. (2007). Association of polymorphisms in odorant binding protein genes with variation in olfactory response to benzaldehyde in Drosophila. Genetics 177, 16551665.CrossRefGoogle ScholarPubMed
Wang, P., Lyman, R. F., Mackay, T. F. C. & Anholt, R. R. H. (2010). Natural variation in odorant recognition among odorant binding proteins in Drosophila melanogaster. Genetics 184, 745758.Google Scholar
Wicher, D., Schäfer, R., Bauernfeind, R., Stensmyr, M. C., Heller, R., Heinemann, S. H. & Hansson, B. S. (2008). Drosophila odorant receptors are both ligand-gated and cyclic-nucleotide-activated cation channels. Nature 452, 10071011.CrossRefGoogle ScholarPubMed
Wong, A. M., Wang, J. W. & Axel, R. (2002). Spatial representation of the glomerular map in the Drosophila protocerebrum. Cell 109, 229241.Google Scholar
Xu, P., Atkinson, R., Jones, D. N. & Smith, D. P. (2005). Drosophila OBP LUSH is required for activity of pheromone-sensitive neurons. Neuron 45, 193200.CrossRefGoogle ScholarPubMed
Yamamoto, A., Zwarts, L., Norga, K., Callaerts, P., Mackay, T. F. C. & Anholt, R. R. H. (2008). Neurogenetic networks for startle-induced locomotion in Drosophila. Proceedings of the National Academy of Sciences of the USA 105, 1239312398.Google Scholar
Yamamoto, A., Anholt, R. R. H. & Mackay, T. F. C. (2009). Epistatic interactions attenuate mutations that affect startle behaviour in Drosophila melanogaster. Genetics Research 91, 373382.Google Scholar
Zhou, S., Stone, E. A., Mackay, T. F. C. & Anholt, R. R. H. (2009). Plasticity of the chemoreceptor repertoire in Drosophila melanogaster. PLoS Genetics 5, e1000681.Google Scholar
Figure 0

Fig. 1. Phenotypic plasticity in the expression of chemoreceptor genes dependent on the physiological state. Relative expression levels of chemoreceptor genes assessed by hybridization of mRNA extracts to cDNA expression microarrays show differences in the expression of four gustatory receptor (Gr), 12 odorant receptor (Or) and 23 odorant-binding protein (Obp) genes between virgin and mated females (a). In contrast, only 17 Obp genes along with Pino, which encodes Pinocchio that resembles an odorant-binding protein (Rollmann et al., 2005), show altered expression in mated compared to virgin males (b). Red bars indicate genes that show altered regulation in both sexes and arrowheads indicate antagonistic regulation between males and females (adapted from Zhou et al., 2009).

Figure 1

Fig. 2. Phenotypic plasticity in the expression of chemoreceptor genes dependent on the developmental stage and sex. Relative expression levels of chemoreceptor genes assessed by hybridization of mRNA extracts to cDNA expression microarrays show differential gene expression between larval and adult life stages. Sexual dimorphism is prevalent among chemoreceptor genes and members of gene clusters are often regulated independently (adapted from Zhou et al., 2009).

Figure 2

Fig. 3. Cluster analysis of chemoreceptor expression across multiple environmental conditions. The chemosensory gene repertoire clusters in 20 relatively small co-regulated transcriptional modules. Note that Obp76a, also known as Lush, and its receptor Or67d group together in module 4 (adapted from Zhou et al., 2009).

Figure 3

Fig. 4. Identifying epistatic interactions among co-isogenic P-element insertion mutants. (a) Diagram of the half-diallel crossing principle. The three sets of the major homologous chromosomes of Drosophila are colour coded with red bars indicating P-element insertion sites. The small fourth chromosome is not depicted. Crosses between a set of homozygous co-isogenic P-element insertion lines (five are shown in this example) allow separation of dominance from non-additive enhancer/suppressor effects. (b) The analysis depicted in (a) can identify ensembles of genes that engage in dynamic epistatic interactions. On the left (green background) is an epistatic ensemble of transposon-tagged genes that affect olfactory behaviour (Sambandan et al., 2006); on the right (orange background) is an epistatic ensemble of transposon-tagged genes that affect startle behaviour (Yamamoto et al., 2008). Overlap between the networks (yellow background) highlights genes that participate in both networks, illustrating pleiotropy.