Do Quantitative Trait Loci (QTL) for a Courtship Song Difference Between Drosophila simulans and D. sechellia Coincide With Candidate Genes and Intraspecific QTL?

doi:10.1534/genetics.166.3.1303

Do Quantitative Trait Loci (QTL) for a Courtship Song Difference Between Drosophila simulans and D. sechellia Coincide With Candidate Genes and Intraspecific QTL?

Jennifer M. Gleason^a and Michael G. Ritchie^a
^a School of Biology, University of Saint Andrews, Saint Andrews, Fife KY16 9TH, Scotland

Corresponding author: Jennifer M. Gleason, 1200 Sunnyside Ave., University of Kansas, Lawrence, KS 66045., jgleason{at}ku.edu (E-mail)

Communicating editor: M. A. F. NOOR

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The genetic architecture of traits influencing sexual isolationcan give insight into the evolution of reproductive isolationand hence speciation. Here we report a quantitative trait loci(QTL) analysis of the difference in mean interpulse interval(IPI), an important component of the male courtship song, betweenDrosophila simulans and D. sechellia. Using a backcross analysis,we find six QTL that explain a total of 40.7% of the phenotypicvariance. Three candidate genes are located in the intervalsbounded by two of the QTL and there are no significant QTL onthe X chromosome. The values of mean IPI for hybrid individualsimply the presence of dominant alleles or epistasis. Becauseunisexual hybrid sterility prevents an F₂ analysis, we cannotdistinguish dominant from additive genetic effects at the scaleof QTL. A comparison with a study of QTL for intraspecific variationin D. melanogaster shows that, for these strains, the QTL wehave identified for interspecific variation cannot be thosethat contribute to intraspecific variation. We find that theQTL have bidirectional effects, which indicates that the geneticarchitecture is compatible with divergence due to genetic drift,although other possibilities are discussed.

THE divergence of mating behaviors influencing sexual isolationplays a fundamental role in speciation. Understanding the geneticarchitecture of courtship is therefore essential for studyingmodels of speciation (SHAW and PARSONS 2002 ). The geneticsunderlying courtship behavior are poorly understood (RITCHIEand PHILLIPS 1998 ), yet the evolution of premating isolationmay be a primary cause of speciation in many taxa (BUTLIN andRITCHIE 1994 ; PANHUIS et al. 2001 ).

The relative importance of different genetic architectures inspeciation has been debated but remains unresolved because ofa lack of empirical evidence (BARTON and CHARLESWORTH 1984 ; CARSON and TEMPLETON 1984 ; BARTON and TURELLI 1989 ; ORRand COYNE 1992 ). Two extreme types of genetic architecturehave been described. Type I architecture is characterized bymany genes of small effect contributing to differences betweenspecies (TEMPLETON 1981 ). In type II architecture, major geneeffects underlie relevant traits. Both architectures dependon the magnitude and direction of allelic effects as well asinteractions among loci. Both conventional crosses and advancesin quantitative trait loci (QTL) analysis allow us to addressthe relative importance of the two types for adaptive traits.Evidence for both type I and type II architectures has beenfound. For example, major gene effects have been reported forpheromonal communication, sexual isolation, and genitalic morphologydifferences in Drosophila (COYNE et al. 1994 ; TRUE et al.1997 ; DOI et al. 2001 ; TAKAHASHI et al. 2001 ). In contrast,acoustical communication has been suggested to have a polygenicmode of inheritance (RITCHIE and PHILLIPS 1998 ; SHAW and PARSONS2002 ; but see HENRY et al. 2002 ).

In addition to the number, type, and genomic placement of genesaffecting behavioral traits, QTL analysis allows assessmentof the potential contribution of candidate genes to the trait.A candidate gene is a gene that is identified through mutationalanalyses as having an effect on the trait. QTL for quantitativetraits, such as Drosophila bristle number, are often concordantwith candidate loci (reviewed in MACKAY 1996 ). However, mutationaleffects may not reflect the same kind of changes that contributeto important natural variation, although polymorphism at a bristlelocus has been shown to affect naturally occurring variation(LAI et al. 1994 ). In general, mutationally defined candidategenes have been implicated in explaining intraspecific variation,but for increasing phylogenetic distance, the candidate geneapproach is less successful (reviewed in HAAG and TRUE 2001).

An additional question that can be addressed through QTL analysisis whether the locations of genes affecting a trait differencebetween species are the same as those for polymorphisms withina species. If the locations are the same, then the same geneticloci may be responsible for trait variability both within andbetween species. Alternatively, intraspecific variants may bedeleterious mutations that have not yet been removed by naturalselection. In that case, intraspecific polymorphisms would notnecessarily be responsible for generating interspecific traitdifferences (NUZHDIN and REIWITCH 2000 ). In studies to date,QTL have been found that are shared within and between species(NUZHDIN and REIWITCH 2000 ; KOPP et al. 2003 ).

Courtship song in Drosophila provides opportunities to studythe genetic architecture of species differences, to determinethe direction of allelic effects, to examine the possible contributionof candidate genes, and to compare intra- and interspecificgenetic architecture. Male Drosophila produce courtship songby wing vibration. Drosophila melanogaster males have two songs:pulse song and hum (or "sine") song. Pulse song consists ofa series of low-frequency, short pulses that affect male andfemale mating behavior. The most important parameter of pulsesong for species recognition in the D. melanogaster group isthe interpulse interval (IPI), that is, the amount of time betweeneach pulse (EWING and BENNET-CLARK 1968 ; RITCHIE et al. 1999). Mean IPI is species specific (KAWANISHI and WATANABE 1980) and has been demonstrated to affect female mating propensityin a species-specific manner (VON SCHILCHER 1976B , VON SCHILCHER1976C ).

In a recent study (GLEASON et al. 2002 ), we examined the geneticarchitecture of D. melanogaster mean IPI with QTL mapping usingrecombinant inbred lines derived from two laboratory strains.Three QTL accounted for 54% of the genetic variation in thetrait. One of the QTL was located on the left arm of the secondchromosome whereas the other two were on the left arm of thethird chromosome. In another QTL study of mean IPI differencebetween D. pseudoobscura and D. persimilis, three QTL explained95.8% of the genetic variation (WILLIAMS et al. 2001 ). Allthree QTL in this latter case were associated with nonrecombiningportions of the X and second chromosomes, so it is possiblethat many genes contribute to each QTL.

Twelve mutationally defined candidate genes are known to affectcourtship song in D. melanogaster. Certain alleles of cacophony(cac), fruitless (fru), paralytic (para), maleless (mle), andslowpoke (slo) affect mean IPI (VON SCHILCHER 1976A , VON SCHILCHER1977 ; WHEELER et al. 1988 ; VILLELLA et al. 1997 ; PEIXOTOand HALL 1998 ). The period (per) locus affects a species-specificcycle in mean IPI, but not the mean itself (KYRIACOU and HALL1980 ), whereas Cysteine string protein (Cys), temperature-induced-paralytic-E(tipE), and slo affect pulse amplitude (PEIXOTO and HALL 1998). Song is completely eliminated with some mutants: doublesex(dsx) alleles eliminate sine song (VILLELLA and HALL 1996 ),whereas some fru alleles eliminate pulse song (WHEELER et al.1988 ; VILLELLA et al. 1997 ). Intrapulse frequency can beaffected by alleles of slo, Cys, and tipE (PEIXOTO and HALL1998 ). The shape of intrapulse cycles is affected by allelesof cac, per, slo, Cys, croaker (cro), transformer (tra), andno-on-or-off-transientA (nonA; VON SCHILCHER 1976A , VON SCHILCHER1977 ; KULKARNI et al. 1988 ; WHEELER et al. 1988 ; BERNSTEINet al. 1992 ; YOKOKURA et al. 1995 ; STANEWSKY et al. 1996). Most of these genes were originally isolated because theyaffect other phenotypes, for example, circadian rhythm (per; KYRIACOU and HALL 1980 ), sex determination pathways (fru,dsx, tra; KULKARNI et al. 1988 ; WHEELER et al. 1988 ; BERNSTEINet al. 1992 ; VILLELLA and HALL 1996 ; VILLELLA et al. 1997), and locomotion (para, slo; PEIXOTO and HALL 1998 ).

The genes identified through mutational analyses serve as possiblecandidate genes for QTL studies of natural variation in thesame traits. In the D. melanogaster study (GLEASON et al. 2002), only tipE fell within a QTL. This does not necessarily meanthat tipE is the gene affecting the trait at this QTL becausemany genes may underlie each QTL. The absence of candidate genesfrom most QTL regions does suggest that the candidate gene approachhas not been successful in identifying the genes underlyingnatural variation in courtship song within these strains ofD. melanogaster.

In this study, we examine the genetic architecture of the differencein mean IPI between D. simulans and D. sechellia. These closelyrelated species differ significantly in their courtship songand form fertile hybrid females. Thus, through QTL backcrossanalyses we can assess the genetic architecture of an importantbehavioral trait in species discrimination (RITCHIE et al. 1999), determine if candidate genes colocalize with QTL for thetrait, identify directional effects to infer the possible roleof drift vs. selection, and determine whether or not QTL responsiblefor intraspecific variability and interspecific differencesfall in locations similar to those found in the D. melanogasterstudy.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Strains and crosses:
One strain each of two species was used in this study. The D.sechellia strain was kindly provided by Jean David. This strain,although probably already inbred, was inbred for a further 18generations of brother-sister mating to produce the line usedin the subsequent crosses. The inbred D. simulans line was kindlyprovided by Jerry Coyne and had five morphological markers,one per chromosome arm (Table 1). Previous studies had shownthat this strain sings with the same mean IPI as wild-type strains(PUGH and RITCHIE 1996 ).

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Table 1. Markers used and their resulting map order

All fly culturing was at 25° and a 12 hr light:12 hr darkcycle using standard techniques. Female D. simulans flies werecrossed to male D. sechellia flies and the female progeny werebackcrossed to D. simulans males. For each cross, one femalewas paired with a single male in a vial (95 x 16.5 mm) for 7days. Multiple crosses were performed to produce 554 males whosesongs were subsequently recorded. In total, 58 crosses and 99backcrosses were used. Using the five morphological markers,we attempted to record songs for all of the 32 backcross phenotypesso that we did not study only the most frequent intraspecificchromosomal combinations.

Courtship song recordings and analysis:
Males were collected on the day of eclosion, genotyped for thefive morphological markers, and isolated in another vial (95x 16.5 mm) until recording. Males were recorded 8–10 daysposteclosion using a custom-built "insectavox" microphone (GORCZYCAand HALL 1987 ) and a Marantz CP430 cassette tape recorder.The male to be recorded, along with a wingless D. simulans orD. sechellia female (the female courted does not influence songparameters, M. G. RITCHIE, unpublished observation), was introducedby aspiration into a mating chamber and recordings were madefor $~$ 5 min from the first burst of pulse song. Temperature wasrecorded as the average of that at the beginning and the endof each recording. Recordings were made between 24.0° and28.1° with a mean of 26.4°. Song was digitized usinga Cambridge Electronic Design 1401 A/D converter (at 2 kHz afterbandpass filtering at $~$ 100 Hz–1 kHz). Individual pulsesof song were detected using an automatic procedure, with subsequentmanual monitoring of data points and song pattern by the experimenter.All analysis used custom-written scripts in the "Spike2" language(Cambridge Electronic Design). Histograms of the IPIs detectedin each recording were examined and the mean IPI value of eachmale entered into the analysis. These procedures have been shownto be accurate for determining mean IPI (RITCHIE and KYRIACOU1994 ).

The number of IPIs obtained for each male recorded ranged from4 to 770. By randomly resampling a selection of songs, we determinedthat at least 30 IPI values were necessary to accurately estimatemean IPI for an individual. Thus, subsequent analyses were performedonly on individuals for which we had at least 30 IPI values.Mean IPI is strongly influenced by temperature (SHOREY 1962). All mean IPI values were corrected to common temperatureof 25° using the formula –1.6(25-T) + I, where T isthe mean temperature of the recording and I is the mean IPIof the recording. The coefficient of 1.6 was empirically derivedfrom other studies (RITCHIE et al. 1994 ; RITCHIE and KYRIACOU1996 ). After temperature correction, four outliers were removedand the data were log transformed to remove a right skew. Variancecomponents reflect the transformed data (i.e., they have notbeen back transformed). Both untransformed and backtransformedeffects are presented (see below). The final sample size forthe quantitative trait was 429 individuals.

Marker scoring:
After recording, males were frozen at –20°. DNA wasisolated from frozen individual males (N = 433) using the methodof GLOOR and ENGELS 1992 . Forty molecular markers were scoredfor each individual (Table 1). These markers were all PCR amplifiedand had different-sized fragments for D. sechellia and D. simulanson 2% agarose, 4% Metaphor agarose (Cambrex), or acrylamidegels. Size differences were caused by natural variation in sequencelength (indels or microsatellites) or by differences in restrictionenzyme sites (Table 1). Hybrids were easily distinguished fromhomozygotes.

Genetic mapping and QTL analysis:
Together with the morphological markers (see above), 45 markerswere scored on 433 individuals. These markers were mapped usingMAPMAKER (LANDER et al. 1987 ). The map obtained was subsequentlyused in QTL analyses using QTL Cartographer version 1.16c (BASTENet al. 1997 ) to map QTL.

Calculation of effects in milliseconds:
Because our data were transformed by natural logs, the resultingeffect of each QTL is dimensionless. The effect, as calculated,is the difference between the mean of the logs for the group(MLG) and the mean of the logs for the traits of all backcrossindividuals (MLT). This difference is equivalent to the logof ratios of the geometric mean for the group (GMG) and thegrand geometric mean (GMT), that is, MLG – MLT = log(GMG/GMT).Therefore, if exp(effect) is multiplied by GMG, the result isGMT. Subtracting GMT from GMG yields the effect in milliseconds.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Marker mapping:
The markers were chosen to have an average spacing of $~$ 6 cM onthe basis of the D. melanogaster map. The average spacing realizedbetween markers was 19.06 cM, because of segregation distortionand our selection for recombinants. Most markers mapped in thesame linear order (Table 1) as in D. melanogaster with the exceptionof a marker pair on the end of the left arm of each chromosome(sc and Pgd on the X chromosome, ex and nt on the second chromosome,and ve and Cdc37 on the third chromosome). In a companion studyof cuticular hydrocarbon QTL in the females derived from thesecrosses, the map order for the X and third chromosomes is thesame as for D. melanogaster, although the order for the secondchromosome is reversed as it is here (J. M. GLEASON, J.-M. JALLON,J. ROUAULT and M. G. RITCHIE, unpublished results). The reversalsare most likely artifacts of being at the end of chromosomes,and as they are not near QTL, the order does not affect theresults. On the right arm of the third chromosome, there isan inversion in D. simulans and D. sechellia relative to D.melanogaster and five markers (Mtn, pros, gl, nos, and e) showthis inversion.

The length of the genetic map found in this study is quite long.Studies of backcross hybrids between D. simulans and D. mauritianahave resulted in maps longer than those of the original species(e.g., LIU et al. 1996 ; TRUE et al. 1997 ). Our long maplength may be derived in part from selection for recombinantindividuals and also from epistatic inviability interactionsamong loci. Genetic incompatibilities leading to inviabilityhave been found in interactions between the X chromosome ofD. sechellia and the autosomes of D. simulans (JOLY et al. 1997; our personal observation). In addition, there was a reductionin viability when the third chromosome was recombinant (JOLYet al. 1997 ). Such interactions will affect observed map lengthsin interspecific studies.

Mean IPI:
The strain of D. simulans had a mean IPI of 56.15 ± 1.699msec and D. sechellia had a value of 67.06 ± 1.789 msec.F₁ hybrid males had a mean IPI value of 50.53 ± 1.090msec. The final data set, of 429 individual, backcrossed males,had a mean IPI value of 50.78 ± 6.331 msec. Evidently,the trait displays dominance for low values of IPI or thereare hybrid incompatibility influences on the trait. Using abackcross design, we cannot distinguish dominant from additivegenetic effects, but because of the sterility of F₁ males, backcrossanalysis is the only crossing scheme possible with these species.

QTL analysis:
The marker on the fourth chromosome (ey) was not significantlyassociated with the trait, and results for this chromosome,which comprises only $~$ 1% of the genome, are not shown. Compositeinterval mapping (CIM) was performed for the rest of the genome.CIM (JANSEN and STAM 1994 ; ZENG 1994 ) combines interval mapping(LANDER et al. 1987 ) with multiple regression. Each intervalflanked by adjacent markers is tested for the presence of aQTL affecting the trait while statistically accounting for theeffects of additional segregating QTL outside the interval.The significance level of P = 0.05 was calculated from 1000permutations of the trait data among marker classes (CHURCHILLand DOERGE 1994 ) and corresponds to a likelihood ratio of 14.029.

Parameters potentially affecting the detection of QTL usingCIM include both the number of background markers used and thesize of the window around the tested interval, within whichlinked markers are excluded from multiple regression. We testeda range of window sizes from 2.5 to 20 cM and found that thewindow size did not influence the results. Forward/backwardstepwise regression resulted in seven significant markers (Table 1)that could be used in CIM. Results varied slightly with theaddition of markers. Fig 1 depicts the results using a backcrossdesign, the Kosambi map function, seven background markers,and a window size of 5 cM. This analysis provides support forthe presence of six QTL that affect mean IPI, four on the rightarm of the second chromosome and two on the right arm of thethird chromosome. The two peaks farthest right on the secondchromosome (QTL 3 and QTL 4, Fig 1) were present in all analysesbut were significant only when four or more markers were includedin the CIM. QTL 1 and QTL 2 were present in all analyses butwere much more significant (likelihood ratio of >50) in analysesusing just one or two markers than in analyses with more markers.The third significant marker (Table 1) is located between QTL3 and QTL 4 and thus has a large effect on the size of thesetwo QTL on the second chromosome.

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Figure 1. Composite interval mapping of the difference in mean IPI between D. simulans and D. sechellia for the three major chromosomes. The positions of the markers are denoted by solid circles along the x-axis. The identity of each marker is given in Table 1. Solid triangles at the top of the graphs indicate the positions of each QTL and are numbered for reference to the text. The significance level at P = 0.05 was determined by 1000 permutations of the data set. The locations of candidate genes are indicated by shaded vertical lines along the x-axis. Abbreviations for candidate genes are given in Table 1.

The two QTL on the third chromosome (QTL 5 and QTL 6) were presentin all analyses and the addition of markers increased the likelihoodscore from $~$ 30, with one marker, to >40, with seven markers.The addition of each marker increased the score. There wereno other significant QTL except in the analysis using just onemarker. In this case, there were two more QTL, one adjacentto QTL 5 and one adjacent to QTL 6. Because the second significantmarker, nanos (Table 1), is positioned between QTL 5 and 6,adding this marker had a large effect on the resolution of QTL5 and 6. For the X chromosome, the analysis with five markersproduced a barely significant QTL at $~$ 0.85 M. Adding in the sixthsignificant marker, located on the far left of the X chromosome,dropped this QTL below significance. Therefore, by using allof the significant markers in the analysis, we are giving aconservative estimate of the number of QTL.

Twelve song candidate genes have been identified in previousstudies. Markers were made for five of these genes and the positionsof the others have been inferred by their location relativeto the markers used (Table 2). Three candidate genes fall withinthe QTL of this study: mle, cro, and fru. In a previous QTLstudy of the mean IPI of D. melanogaster, a different candidategene, tipE, fell within a QTL (GLEASON et al. 2002 ). None ofthe six QTL from this study overlaps with the three QTL of theprevious study.

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Table 2. Song candidate genes

All the QTL on the second chromosome had a negative additiveeffect whereas those on the third chromosome had a positiveadditive effect, with respect to D. simulans (Table 3). In total,the QTL explain 40.66% of the phenotypic variance and rangeindividually from 3.44 to 9.38%. The magnitude of the QTL rangedfrom 22.1 to 36.8% of the phenotypic difference between theparents. If a threshold of >25% of the phenotypic variance explainedis used to designate a major QTL (BRADSHAW et al. 1995 , BRADSHAWet al. 1998 ), then the trait here is not influenced by majorQTL.

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Table 3. QTL locations and effects

DISCUSSION

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

QTL studies of interspecific differences in adaptive quantitativetraits have found QTL with both large (LAURIE et al. 1997 ; MACDONALD and GOLDSTEIN 1999 ) and minor effects (e.g., FISHMANet al. 2002 ). Many interspecific trait differences have beenshown to be polygenic (e.g., KIM and RIESEBERG 1999 ; ZENGet al. 2000 ) and it has been hypothesized that the time sincespecies divergence is positively correlated with the numberof QTL found (KIM and RIESEBERG 1999 ). In the present study,none of the QTL for mean IPI identified has a major effect andthe majority of the phenotypic variation is not explained, indicatingthat the study lacked sufficient resolution to detect additionalsmall-effect QTL that also influence this trait difference.This is in contrast to the study of D. melanogaster in whichmajor QTL were found for the same trait (GLEASON et al. 2002). Overall, the difference in QTL effect between the studiesfollows the KIM and RIESEBERG 1999 hypothesis, because thedivergence between species (D. simulans and D. sechellia) isgreater than that between D. melanogaster strains. The parentallines for the intraspecific study did not differ significantlyfor mean IPI, and the QTL reflect transgressive segregation(GLEASON et al. 2002 ). Differences in the time scales of withinvs. between species comparisons will confound conclusions concerningthe nature of genotypic differences within species and thosecontributing to speciation (WU and HOLLOCHER 1998 ). Our dataare compatible with the suggestion that the large-effect QTLof the within-species study reflect recent mutations at deleteriousgenes that have not yet been fixed, whereas between-speciesdifferences arise over a much longer timescale and are thereforemore likely to reflect numerous QTL of more minor effect (ORR1998A ).

The greater absolute trait values for between-species divergencethan for within-species variation could mean that genes of similarabsolute effect on the trait would appear as major-effect genesin one study and as minor-effect genes in another. In this study,effects range from 2.41 to 4.02 msec, whereas for the D. melanogasterstudy (GLEASON et al. 2002 ) effects ranged from 0.56 to 0.826msec. The nature of the genes involved is thus not conclusivelydifferent within and between species, because our minor-effectgenes explain a greater absolute value of the trait than dothe major-effect genes found within species.

Our interspecific QTL are different from the intraspecific QTLof D. melanogaster. For D. melanogaster, one QTL was on theleft arm of the second chromosome and two were on the left armof the third chromosome. In the present study, all QTL are onthe right arms of the second and third chromosomes (Fig 1, Table 3). Thus, the QTL for intraspecific variation and intraspecificdifferences for mean IPI are located on different chromosomearms. This result differs from others for morphological traits(NUZHDIN and REIWITCH 2000 ; KOPP et al. 2003 ) in which intraspecificand interspecific traits are sometimes affected by overlappingQTL. Because the study of D. melanogaster QTL is only for asingle pair of strains, many other QTL might be implicated inother crosses of different populations, but our results do confirmthat there are many loci with the potential to influence IPI.

Comparisons of these QTL locations to other quantitative geneticsstudies of song loci are difficult. PUGH and RITCHIE 1996 ,in a low-resolution study of the difference in IPI between D.simulans and D. mauritiana, found contributions of all of thechromosome arms. For the D. pseudoobscura and D. persimiliscomparison (WILLIAMS et al. 2001 ), QTL were found in the invertedregions of the X chromosome (equivalent to the D. melanogasterX and 3L; POWELL 1997 ) and the second chromosome (equivalentto D. melanogaster 3R). There is potential overlap between ourQTL 5 and 6 with the D. pseudoobscura and D. persimilis X chromosomeQTL; however, lack of common markers between the two studiesprecludes exact comparisons. In addition, the large bias ininterspecies gene flow between these two species in uninvertedareas of the genome (MACHADO and HEY 2003 ) makes the comparisonbetween species groups uninformative. YAMADA et al. 2002 founda large effect of the second chromosome on song differencesbetween D. anannassae and D. pallidosa. Although the D. anannassaesecond chromosome is equivalent to the third chromosome of D.melanogaster (POWELL 1997 ), the resolution of those loci isnot sufficient to determine whether the same genes might beinvolved in this study.

Three candidate loci for song fall within the interspecificQTL. Two of these candidate genes, mle and fru, have allelesthat affect mean IPI in D. melanogaster (VILLELLA et al. 1997; PEIXOTO and HALL 1998 ). The third gene, croaker, causespolycyclic pulses (YOKOKURA et al. 1995 ). Presence within aQTL interval does not confirm that the candidate gene is involvedin the trait because many genes underlie the QTL regions, butfinding that a candidate gene underlies a QTL indicates thatthese genes are worth examining further for interspecific differentiation.Four of the six QTL detected do not contain candidate genes.

In the study of QTL for D. melanogaster mean IPI (GLEASON etal. 2002 ), a different candidate gene was implicated; the gene,tipE, influences song amplitude and intrapulse frequency (PEIXOTOand HALL 1998 ). The other two QTL did not coincide with candidategenes. Thus, at one level, the candidate gene approach has notbeen successful for identifying genes affecting natural variationin mean IPI within or between species. If candidate genes influencegenetic variability in natural populations, we would expectthem to be equally likely to contribute to within- and between-speciesdifferences, unless variability was transient due to selection,in which case they would be more likely to be detected in interspecificanalyses. Other studies have clearly demonstrated that candidategenes can influence natural variation between species (e.g., SUCENA and STERN 2000 ; HAAG and TRUE 2001 ), including studiesof Drosophila song (KYRIACOU 2002 ). Interestingly, the nonAgene has been shown to influence interspecific differences incourtship song when introgressed from D. melanogaster to D.virilis (CAMPESAN et al. 2001 ), but natural variation at thislocus within and among D. virilis group species does not correlatewith song variation (HUTTENEN et al. 2002 ). Most mutants atsuch genes might be rapidly eliminated by strong selection.

The genetic architecture of species differences may give insightsinto the speciation process. We have found that a type I geneticarchitecture (many small-effect genes) underlies the mean IPIspecies difference. Combined with the bidirectional alleliceffects, our data are most compatible with a history of gradualdivergence without strong selection, possibly by drift (ORR1998B ; SHAW and PARSONS 2002 ). Directional selection mightbe expected, given that the trait is sexually dimorphic, isunder selection from female mating preferences, and contributesto sexual isolation (RITCHIE et al. 1998 ). However, if preferenceswere stabilizing or often changed direction (under an unstableFisherian scenario, for example), drift might still predominatein the long term. In addition, as these species have a longhistory of allopatry (although D. simulans has recently beenintroduced to the Seychelles), character displacement is unlikelyto have generated consistent directional selection.

ACKNOWLEDGMENTS

For technical help with scoring markers, we thank Tanya Hamilland Carrie Adamson. Rosemary Bevan assisted with Drosophilaculturing and Terry Gleason provided statistical advice. Wethank Maria Orive, Anne Danielson-François, Tara Marriage,John Kelly, members of the Kelly Lab, Mohamed Noor, and twoanonymous reviewers for comments on the manuscript. This workwas supported by a grant (GR3/10786) from the Natural EnvironmentResearch Council (UK) to M.G.R.

Manuscript received October 1, 2003; Accepted for publication December 6, 2003.

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

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