Candidate Quantitative Trait Loci and Naturally Occurring Phenotypic Variation for Bristle Number in Drosophila melanogaster: The Delta-Hairless Gene Region

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Candidate Quantitative Trait Loci and Naturally Occurring Phenotypic Variation for Bristle Number in Drosophila melanogaster: The Delta-Hairless Gene Region

Richard F. Lyman^a and Trudy F. C. Mackay^a
^a Department of Genetics, North Carolina State University, Raleigh, North Carolina 27695

Corresponding author: Trudy F. C. Mackay, Department of Genetics, Box 7614, North Carolina State University, Raleigh, NC 27695, trudy_mackay{at}ncsu.edu (E-mail).

Communicating editor: P. D. KEIGHTLEY

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Delta (Dl) and Hairless (H) are two chromosome 3 candidate neurogenicloci that might contribute to naturally occurring quantitativevariation for sensory bristle number. To evaluate this hypothesis,we assessed quantitative genetic variation in abdominal andsternopleural bristle numbers among homozygous isogenic thirdchromosomes sampled from nature and substituted into the Samarkand(Sam) inbred chromosome 1 and 2 background; among homozygouslines in which the wild-derived Dl-H gene region was introgressedinto the Sam chromosome 3 background; and among Dl-H regionintrogression lines as heterozygotes against the Sam wild-typestrain and derivatives of Sam into which mutant Dl and H alleleshad been introgressed. Variation among the Dl-H region introgressionlines accounted for 36% (8.3%) of the total chromosome 3 amongline variance in abdominal (sternopleural) bristle number andfor 53% of the chromosome 3 sex x line variance in abdominalbristle number. Naturally occurring alleles in the Dl-H regionfailed to complement a Dl mutant allele for female abdominalbristle number and sternopleural bristle number in both sexes,and an H mutant allele for both bristle traits in males andfemales. These results are consistent with the hypothesis thatnaturally occurring alleles at Dl and H contribute to quantitativegenetic variation in sensory bristle number.

MOST phenotypic differences between individuals, such as variationin anatomical dimensions, behavior, and susceptibility to disease,are quantitative in nature, of degree rather than kind (FALCONERand MACKAY 1996 ). Phenotypic variation of quantitative traitsis characterized by the simultaneous segregation of allelesat multiple loci, the effects of which are sensitive to theenvironment. A major challenge in medicine, plant and animalbreeding and evolution is to determine at what genetic lociallelic variation contributes to phenotypic variation in quantitativetraits, and to estimate the effects of the segregating alleles.This task is not simple, because the allelic effects at eachlocus are, by definition, too small to be perceived over andabove the background noise of segregation of other alleles affectingthe trait of interest and environmental variation. Quantitativetrait loci (QTLs) can now be mapped in many species by linkageto polymorphic, neutral molecular markers (reviewed by TANKSLEY1993 ). However, even with dense molecular marker maps, it isdifficult to localize QTLs to regions much smaller than a fewcM with initial whole genome screens, as informative recombinationevents between closely linked loci become increasingly rareand require prohibitive sample sizes to recover. Although sufficientlyprecise for utilizing the QTL in a selective breeding program,for example, this level of resolution is still several ordersof magnitude away from identifying allelic differences at asingle locus responsible for variation in a quantitative traitphenotype.

The most promising approach for proceeding from QTL to geneticlocus is to search for candidate genes in the region to whichthe QTL maps. Candidate loci can be proposed a priori, basedon functional relationships of known genes to the trait phenotype(i.e., loci in the biochemical or developmental pathways leadingto the phenotype of interest), or, with considerably more difficulty,from positional cloning subsequent to high-resolution meioticmapping. Underlying the candidate gene approach is the assumptionthat variation in quantitative traits is caused by the segregationof "isoalleles" with small effects at loci previously identifiedby alleles with major effects (THOMPSON 1975 ; MACKAY 1985; ROBERTSON 1985 ). Obvious limitations of the candidate locusapproach are that all of the loci involved in the relevant biochemicalor developmental pathways leading to the phenotype of interestare usually not known, and loci that are not obvious candidatesmay have undescribed and unexpected pleiotropic effects on thetrait.

Although roughly concordant map positions of QTLs and candidateloci from an initial mapping population suggest a testable hypothesis,several criteria need to be fulfilled before it can be acceptedthat the candidate gene and the QTL are one and the same. (1)If "near-isoallelic" or congenic strains, in which alternativealleles of the QTL are introgressed into a common background,can be established, variation among the near-isoallelic linesconfirms the presence of loci affecting the trait, includingthe candidate locus, in the introgressed gene region (DOEBLEYet al. 1995 ; ESHED and ZAMIR 1996 ). In the absence of homologousrecombination, the precision of this analysis is limited bythe length of the introgressed fragment containing the QTL.(2) Quantitative complementation of QTL alleles with a majormutation and a standard wild-type allele at the candidate locustests for genetic interaction between the QTL alleles and knownalleles at the candidate locus (LONG et al. 1996 ; MACKAY andFRY 1996 ). This test is not definitive, because observed interactionscould be allelic or epistatic, and failure to observe interactionmay be due to interallelic complementation. (3) If the candidategene has been cloned and characterized at the molecular level,population-level association studies of molecular variationin the candidate gene and phenotypic variation in the quantitativetrait can implicate the candidate locus as a QTL (e.g., SINGet al. 1988 ; MACKAY and LANGLEY 1990 ; CORDER et al. 1993; LAI et al. 1994 ). A strong association of a molecular polymorphismin a candidate gene with phenotypic variation could arise ifthe polymorphism causes the phenotypic variation, in which casethe association will be found in all populations with that particularmolecular variant. However, a strong association could alsobe found if the molecular variants are in linkage disequilibriumwith the true causal polymorphism. In the latter case, conflictingresults may be obtained from independent studies in differentpopulations due to differences in population history, and misleadinglinkage disequilibria can arise from recent admixture of populationswith different frequencies of molecular variants in the candidategene region and different average phenotypes for the trait ofinterest. Further, sorting out which of the many nucleotideand length polymorphisms throughout the regulatory and codingsequences of the candidate gene are functional and which arephenotypically neutral is a nontrivial task. (4) In geneticallytractable organisms, it should be possible to demonstrate functionalcomplementation of a null mutation at the candidate locus withthe QTL allele in transgenic individuals. Whether transgenicrescue of a null allele can be used to identify the molecularpolymorphism(s) that differentiate alternative QTL alleles probablydepends on the availability of targeted gene replacement, becauseposition effects of randomly integrated transgenes on the traitmight be as large as the QTL effects themselves (MACKAY et al.1992A ; LYMAN et al. 1996 ). (5) Finally, if naturally occurringvariation at a candidate gene causes phenotypic variation ina quantitative trait, it follows that spontaneous mutationsat the candidate locus should have phenotypic effects on thetrait. The converse is not necessarily true; loci at which spontaneousmutations affect the quantitative trait phenotype may not contributeto naturally segregating variation if functional variation inthe gene decreases fitness.

The above map position, genetic complementation, allelic associationand mutation detection criteria are not individually sufficientproof that a candidate gene is the genetic locus correspondingto a QTL. The case becomes stronger if multiple independentpieces of evidence point to the verity of this hypothesis. Forthis reason, comprehensive evaluations of the extent to whichallelic variation at candidate loci contributes to quantitativegenetic variation may be restricted to quantitative traits inmodel organisms for which the entire repertoire of genetic testsis feasible. One such model system is the number of sensorybristles of Drosophila melanogaster. Drosophila abdominal andsternopleural bristle numbers are highly genetically variable,with heritabilities of ~0.5 (FALCONER and MACKAY 1996 ). Bristlenumbers have historically been used to elucidate basic quantitativegenetic principles such as short- (CLAYTON et al. 1957 ; FRANKHAMet al. 1968 ) and long-term (CLAYTON and ROBERTSON 1957 ; JONESet al. 1968 ) response to selection; selection limits (YOO 1980A); spontaneous mutation rates (reviewed by KEIGHTLEY et al.1993 ; HOULE et al. 1996 ); the effects of recombination (MCPHEEand ROBERTSON 1970 ), population structure (MADALENA and ROBERTSON1975 ) and environmental heterogeneity (MACKAY 1981 ) on geneticvariation and response to selection; and the chromosomal locations,numbers and effects of QTLs contributing to selection response(BREESE and MATHER 1957 ; THODAY 1979 ; SHRIMPTON and ROBERTSON1988A , SHRIMPTON and ROBERTSON 1988B ; LONG et al. 1995 ).As Drosophila bristles are sensory organs of the peripheralnervous system, appropriate candidate loci for bristle numberQTLs are the many genes that are involved in the developmentof the nervous system and sensory organs (CAMPOS-ORTEGA 1993; JAN and JAN 1993 ). Other candidate bristle number QTLs areloci with major mutant effects on bristle number that have not(yet) been implicated in the bristle development pathway.

Several lines of evidence are consistent with the hypothesisthat quantitative variation in bristle number is at least partlyattributable to variation in candidate bristle loci. (1) QTLsresponsible for the divergence between high and low selectionlines map to approximately the same positions as several candidatebristle development loci (SHRIMPTON and ROBERTSON 1988B ; LONGet al. 1995 ). (2) Naturally occurring (LONG et al. 1996 ) andspontaneous mutant (MACKAY and FRY 1996 ) high and low allelesat bristle number QTLs genetically interact with mutations atcandidate bristle number loci. (3) Molecular variation at candidateneurogenic loci is associated with naturally occurring phenotypicvariation in bristle number (MACKAY and LANGLEY 1990 ; LAIet al. 1994 ). (4) Occasionally, alleles at candidate bristleloci with large effects are found segregating at low frequencyin natural populations (MCBRIDE and ROBERTSON 1963 ; FRANKHAMand NURTHEN 1981 ). (5) Spontaneous mutations at candidate bristlenumber genes have contributed to long-term artificial selectionresponse (HOLLINGDALE 1971 ; FRANKHAM et al. 1978 ; FRANKHAM1980 ; YOO 1980B ). (6) P-element insertional alleles at neurogenicloci have quantitative phenotypic effects on bristle number(LYMAN et al. 1996 ).

Although these observations collectively support the hypothesisthat genetic variation at known bristle loci contributes toquantitative variation in bristle number, they are neverthelessa somewhat eclectic set of data in that the various steps ofthe proof are illustrated by different candidate loci. To systematicallyevaluate the extent to which variation at candidate genes contributesto quantitative genetic variation for bristle number in general,it is necessary to collect information on QTL map position,genetic and functional complementation, allelic associationand mutational analysis for a sample of several candidate loci.In this way, we can begin to disperse the statistical "fog"surrounding at least one model quantitative trait and beginto describe quantitative variation in terms of defined molecularvariants, their frequencies, and allelic effects (ROBERTSON1967 ). We have begun such a comprehensive investigation witha quantitative and molecular genetic analysis of naturally occurringvariation in the Delta (Dl) gene region.

The Drosophila peripheral nervous system (PNS) is progressivelydetermined by a number of interacting genes. Initially, theproneural genes endow small clusters of cells with the potentialto become neuronal precursors, after which the neurogenic locisingle out a subset of cells in the proneural cluster to becomeneuronal precursors (CAMPOS-ORTEGA 1993 ; JAN and JAN 1993). Subsequent steps in the development of the PNS are the commitmentof neuronal precursors, specification of identity of neuronalprecursors, and sensory organ cell fate specification (JAN andJAN 1993 ). Of the many loci known that control each step inthe pathway (JAN and JAN 1993 ), interactions of the neurogenicloci during the process of lateral specification of neuronalprecursors is particularly well established (ARTAVANIS-TSAKONASet al. 1995 ). Neuronal precursor cell fate is specified byinteractions between proteins of the Notch signaling pathway.The eponymous Notch (N) gene encodes a transmembrane receptorprotein, and Dl encodes a transmembrane protein that is an extracellularligand for Notch; Delta is thought to activate the Notch receptorby binding of the epidermal growth factor-like repeats of bothmolecules (ARTAVANIS-TSAKONAS et al. 1995 ). The Hairless (H)gene is closely linked to Dl and interacts genetically withboth N and Dl (LINDSLEY and ZIMM 1992 ). It encodes a nuclearprotein (MAIER et al. 1992 ) that is thought to act at one ofthe later stages in PNS development (JAN and JAN 1993 ; ARTAVANIS-TSAKONASet al. 1995 ).

Previously, we mapped one of five chromosome 3 QTLs responsiblefor the divergence of abdominal bristle number between artificialselection lines, derived from a natural population, to cytogeneticinterval 89D-92E, which includes both Dl (92A1-2) and H (92E12-14; MAIER et al. 1992 ; LONG et al. 1995 ). The effect of thisinterval was 3.0 abdominal and 1.4 sternopleural bristles, averagedover sexes, and it accounted for 22% (30%) of the third chromosomedivergence in abdominal (sternopleural) bristle number. Mutationsat Dl and H showed strong genetic interactions with high andlow selection line chromosomes (LONG et al. 1996 ); further,mutations at Dl and H interact with spontaneous mutations affectingabdominal and sternopleural bristle number (MACKAY and FRY 1996). Although implicating segregating and mutational variationat Dl and H as contributing to quantitative genetic variationin bristle number, these studies are subject to the caveatsthat the QTL map position needs to be confirmed independentlyand that the genetic interactions observed between high andlow selection lines (or whole chromosomes from selection lines)and the Dl and H mutant alleles might not be allelic. Here,we have constructed near-isoallelic lines of the Dl-H gene regionfor a sample of unselected chromosomes from the same naturalbase population used to establish the selection lines of LONGet al. 1995 , and we demonstrate that QTLs in this region bothcontribute to quantitative variation in bristle number and failto complement Dl and H mutant alleles. In the companion article(LONG et al. 1998 ), we provide further evidence that Dl isa genetic locus at which segregating variation contributes toquantitative variation in bristle number from associations betweenmolecular variation at Dl and phenotypic variation in bristlenumber.

MATERIALS AND METHODS

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ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

All Drosophila stocks were reared in shell vials with 10 mlcornmeal-agar-molasses medium, at 25°. For details of theloci and balancer chromosomes used, see LINDSLEY and ZIMM 1992.

Chromosome 3 substitution lines:
Gravid D. melanogaster females were obtained from the Raleigh,NC, Farmer's Market in 1988 and used to establish isofemalelines. This sample of isofemale lines was used to establishthe base population from which the artificial selection linesfor abdominal bristle number used in QTL mapping were derived(LONG et al. 1995 ). In addition, a single third chromosomewas extracted from each of 63 of these isofemale lines and substitutedinto the genetic background of the highly inbred Sam; ry⁵⁰⁶strain (see LYMAN et al. 1996 ) by standard techniques usingbalancer chromosomes (MACKAY et al. 1996 ). The genotype ofthese lines was thus Sam1; Sam2; C3i, where i = 1, 2, ... ,63 wild-derived third chromosomes.

Abdominal bristle number (the number of hairs on the most-posteriorsternite; segment six of females and segment five of males)and sternopleural bristle number (the sum of the number of bristleson the right and left sternopleural plates) were recorded on10 C3i males and females in each of two replicate vials perline (i.e., 63 lines x two vials/line x two sexes/vial x 10individuals/sex = 2520 individuals).

Construction of Dl-H region introgression lines:
An allele of the Delta (Dl³, 3-66.2) locus was substituted intothe Sam; ry⁵⁰⁶ background by 20 generations of backcrossingDl³ heterozygous females to Sam; ry⁵⁰⁶ males. This backcrosschromosome (Dl³ BC20) was subsequently maintained balanced againstTM3, Sb ry^RK, in a stock of genotype Sam1; Sam2; Dl³ BC20/TM3,Sb ry^RK.

Let C3i refer to the wild isogenic third chromosomes in theSam background, and Dl³ BC20/Sb to the strain with the balancedDl allele in the Sam background. At G0, C3i females were crossedto Dl³ BC20/Sb males in two replicate vials per line. At G1,C3i/Dl³ BC20 females were backcrossed to Dl³ BC20/Sb males,keeping the two replicate backcrosses per line distinct. Thiscross was repeated for nine further generations. After 10 backcrossgenerations, the introgressed C3i regions should contain thewild alleles at the Dl locus plus a linked segment of wild-derivedchromosome ~10 cM on either side of Dl (CROW and KIMURA 1970, pp. 94–95). Keeping two independent backcross lines ofeach wild chromosome controls for variation in the size of theintrogressed fragment, as variation in bristle number amongintrogression lines can be partitioned into that common to theindependent backcross lines and that between replicate backcrosslines, which is attributable to variation in flanking chromosomefragments (see below). Because the Hairless (H) locus at 3-69.5is only 3.3 map units away from Dl, it is likely that the introgressedregions also contain wild-type H alleles. Therefore, we referto the genotype of the introgression lines as Dl-Hi. At G11,Dl³ BC20/Dl-Hi males from each independent backcross line werecrossed to Dl³ BC20/Sb females. Sb/Dl-Hi females and males weremated inter se at G12, and at G13 Dl-Hi homozygous females andmales were crossed to establish the Dl-H region introgressionlines. There were a total of i = 62 pairs of introgression lines(one of the original isogenic third chromosomes did not survivethe entire backcross procedure), of which 59 were homozygousviable.

Homozygous effects, Dl-H region:
Abdominal and sternopleural bristle numbers were recorded for10 Dl-Hi males and females in each of two replicate vials perbackcross replicate, that is, 59 lines x two backcrosses/linex two vials/backcross x two sexes/vial x 10 individuals/sex= 4720 individuals.

Heterozygous effects, Dl-H region:
Heterozygous effects of the 62 Dl-Hi introgression lines weredetermined against three strains: (1) the Sam; ry⁵⁰⁶ straininto which background the wild third chromosomes had been introgressedand which contain a wild-type allele at the Dl and H loci (simplyabbreviated Sam below); (2) the Sam; Dl³ BC20 strain with anextreme Dl mutation and a wild-type allele of H (abbreviatedDl³ below); and (3) Sam; H BC20, constructed by 20 generationsof backcrossing H to Sam; ry⁵⁰⁶ (MACKAY and FRY 1996 ), whichcontains the mutant H allele and a wild-type Dl allele (abbreviatedH below). Abdominal and sternopleural bristle numbers of thethree heterozygous genotypes were recorded for 10 males andfemales in each of two replicate vials per backcross replicate,that is, 62 lines x two backcross replicates/line x two replicatevials/backcross x two sexes x 10 individuals/sex = 4960 individualsper heterozygous genotype.

Quantitative complementation effects:
Complementation tests typically involve recessive mutationswith large phenotypic effects, so the heterozygote between thestrain containing a putative mutation (m*) interacting withthe locus of interest and the strain containing a recessivemutation at the tested locus (m) can be unambiguously classifiedas mutant or wild type. The logic of complementation testingcan be extended to alleles with small, quantitative and additive(i.e., not completely recessive) effects by recognizing thatthe traditional test is for a difference in heterozygous effectbetween m*/+ and m*/m genotypes. That is, failure to complementis inferred if the degree of dominance of m* changes accordingto whether the allele at the locus tested is mutant or wildtype. Therefore, the analogous test for genetic interactionbetween a wild-derived allele affecting bristle number in aDl-H introgression line and Dl³ or H is the difference in bristlenumber between either Dl-Hi/Dl³ or Dl-Hi/H (the Tester crosses)and Dl-Hi/Sam (the Control cross) genotypes. However, becausethe Dl³ and H mutations themselves have heterozygous effectson bristle number (MACKAY and FRY 1996 ) and the chromosomescontaining these mutations have linked non-Sam genomic fragmentsthat might also have heterozygous effects on bristle number,a difference in bristle number between Tester and Control genotypesfor any one introgression line is uninformative. However, variationin the Tester-Control difference among lines is indicative ofvariation in degree of dominance of the Dl-H introgressed regionsas heterozygotes against wild-type and mutant alleles at candidateloci and is interpreted as quantitative failure to complement.Formally, variation in Tester-Control bristle number effectsis detected as a significant cross by line interaction termby analysis of variance.

Statistical analyses:
The whole chromosome 3 homozygote bristle number data were analyzedby two-way factorial analysis of variance (ANOVA), with sex(fixed) and line (random) cross-classified main effects andreplicate vial a random effect nested within lines. Sums ofsquares were partitioned into sources (degrees of freedom) attributableto Sex, S (1), Line, L (62), S x L (62), Replicate, R(L) (63),S x R(L) (63) and Error, E (2268). The homozygous and heterozygousDl-H region bristle number data were analyzed similarly by two-wayfactorial ANOVA, with sex and line cross-classified main effects,backcross replicate a random effect nested within lines andreplicate vials nested within (line x backcross). Sums of squares(degrees of freedom) were partitioned into sources attributableto S (1), L (58), S x L (58), Backcross, BC(L) (59), S x BC(L)(59), R(L x BC) (118), S x R(L x BC) (118) and E (4248) forthe homozygous introgression lines and to S (1), L (61), S xL (61), Backcross, BC(L) (62), S x BC(L) (62), R(L x BC) (124),S x R(L x BC) (124) and E (4464) for the heterozygous introgressionlines. Analyses of the quantitative complementation test dataincluded the effect of Cross (C) as an additional fixed, cross-classifiedmain effect. Thus, sums of squares were partitioned by three-wayfactorial ANOVA into sources (degrees of freedom) attributableto C (1), S (1), C x S (1), L (61), C x L (61), S x L (61),C x S x L (61), BC(L) (62), C x BC(L) (62), S x BC(L) (62),C x S x BC(L) (62), R(C x L x BC) (248), S x R(C x L x BC) (248)and E (8928). All ANOVAs and tests of significance were calculatedusing the Proc GLM procedure in SAS (SAS Institute, Inc., Cary,NC). Variance component estimation was done using SAS Proc VARCOMP.Linear regressions and correlations of line means were computedusing the SAS procedures Proc REG and Proc CORR, respectively.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Distribution statistics:
Quantitative variation in abdominal and sternopleural bristlenumbers was assessed among (1) 63 isogenic third chromosomes,sampled from the Raleigh natural population and substitutedinto the common inbred Sam strain background; (2) homozygousnear-isoallelic lines, in which the Dl-H gene region from theRaleigh third chromosomes was introgressed into the Sam thirdchromosome background; and (3) near-isoallelic Dl-H gene regionlines as heterozygotes against the wild-type Sam strain andcongenic derivatives of Sam into which mutant Dl³ and H alleleshad been introgressed. The distribution statistics of line meansare given in Table 1. The mean bristle number is much greater(less) in the backcross lines heterozygous for Dl (H) mutantalleles than in the backcross homozygotes, consistent with thedominant loss-of-function effects of these alleles. As is commonlyobserved, females have more bristles than males, across allgenotypes. The variance among homozygous Dl-H region line meansis considerably reduced relative to the whole chromosome 3 homozygotesfor both bristle traits (Figure 1), as expected if there aremultiple QTLs affecting bristle number on chromosome 3 and ifbackcrossing to a common inbred strain has been successful.The variance among heterozygous introgression line means isgenerally less than that among homozygous Dl-H region lines,with the interesting exceptions of female abdominal bristlenumber in crosses to Dl³ and sternopleural bristle number forboth sexes in crosses to H. These observations are discussedin detail below. The line means are for the most part normallydistributed.

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Figure 1. —Distributions of mean abdominal and sternopleural bristle number among homozygous whole chromosome 3 substitution lines (Raleigh C3) and among homozygous Dl-H region introgression lines derived from them. Solid bars are for male, and open bars for female line means.

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Table 1. Distribution statistics of abdominal (AB) and sternopleural (ST) bristle number line means

Chromosome 3 substitution lines:
The variance components ( ${sigma}$ ²) and results of tests of significancefrom analyses of variance of bristle number among the chromosome3 substitution lines are given in Table 2. The main effectof Sex was highly significant for abdominal bristle number butnot for sternopleural bristle number in this set of lines, indicatingsexual dimorphism for the former trait (Table 1) but not thelatter. There was highly significant variation among lines forboth bristle traits, indicating substantial naturally occurringgenetic variation for bristle number. The S x L interactionterm was highly significant for abdominal bristle number andmarginally significant for sternopleural bristle number. Theinterpretation of the significant S x L interaction is thatthe female-male difference in bristle score varied among thelines, that is, there was significant genetic variation forsexual dimorphism for bristle traits, particularly for abdominalbristle number.

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Table 2. Variance components ( ${sigma}$ ²) and significance of mean squares (P) from analyses of variance of bristle number for isogenic chromosome 3 substitution lines

Estimates of the genetic variance (V_G) and heritability (h²)for abdominal and sternopleural bristle number attributableto chromosome 3 can be obtained from the estimates of variancecomponents given in Table 2. Because these lines are inbred,the variance component among lines ( ${sigma}$ ²_L ) estimates 2FV_G, andthe S x L variance component ( ${sigma}$ ²_SL ) estimates 2F(1/2V_G), assuminga strictly additive model (FALCONER and MACKAY 1996 ). For completelyhomozygous lines, F = 1; thus, the genetic variance of bristlenumber was estimated by ${sigma}$ ²_{L +}²_SL . The estimates of V_G attributableto variation among isogenic third chromosomes extracted fromnature were 2.38 for abdominal bristle number and 2.72 for sternopleuralbristle number. Taking the error variance, ${sigma}$ ²_E, as the estimateof the environmental variance, V_E, the heritability of bristlenumber was calculated from h² = V_G/(V_G + V_E). The estimateswere h² = 0.39 for abdominal bristle number and h² = 0.48 forsternopleural bristle number. HOULE 1992 has argued that itis appropriate for many purposes to scale genetic and environmentalvariances by the mean and recommends computing the coefficientsof genetic (CV_G) and environmental (CV_E) variance as and ,respectively, where is the mean value of the trait. For thesedata, = 21.4 for both abdominal and sternopleural bristle numbers.Therefore, CV_G = 7.2 for abdominal bristle number and 7.7 forsternopleural bristle number, and CV_E = 9.1 for abdominal bristlenumber and 8.0 for sternopleural bristle number. Whether expressedas h² or CV_G and CV_E, these estimated quantitative genetic parametersfor the two bristle traits are typical of previous whole genomeestimates that have been obtained for these traits in otherpopulations using different experimental designs (e.g., ROFFand MOUSSEAU 1987 ; HOULE 1992 ; FALCONER and MACKAY 1996).

Homozygous effects, Dl-H region:
The Dl gene region from the isogenic third chromosome lineswere introgressed into a common inbred chromosome 3 backgroundby 10 generations of backcrossing, with two independent backcrossesper line. These lines are expected to contain, on average, 20cM of wild-derived genome flanking the Dl locus and are thusexpected to be co-isogenic for 90 cM/110 cM = 82% of the thirdchromosome, or 276 cM/296 cM = 93% of the entire genome, where110 cM and 296 cM are the approximate map lengths of the thirdchromosome and the entire genome, respectively (LINDSLEY andZIMM 1992 ).

The results of analysis of variance of abdominal and sternopleuralbristle numbers among the Dl-H region homozygous introgressionlines are given in Table 3. The main effect of Sex was significantin these and all other analyses of these lines and indicatessexual dimorphism for both bristle traits (Table 1). This commonobservation will not be considered further. There was significantvariation for abdominal and sternopleural bristle numbers amongintrogression lines, indicating segregating variation at lociaffecting these traits in this region of the genome. For abdominalbristle number, 1.090/3.018 = 36.1% of the total chromosome3 variance among lines was attributable to variation in theDl-H region, whereas only 8.3% (0.435/5.233) of the variationamong whole chromosome 3 lines for sternopleural bristle numberwas attributable to genetic variation in the Dl-H region. Theseobservations are consistent with those from mapping studiesthat showed multiple factors on the third chromosome affectedresponse to artificial selection for abdominal (LONG et al.1995 ) and sternopleural (M. C. GURGANUS, S. V. NUZHDIN andT. F. C. MACKAY, unpublished results) bristle numbers from theRaleigh base population. There was also significant S x L variationfor abdominal bristle number among the Dl-H region introgressionlines, accounting for 0.460/0.869 = 52.9% of the S x L variationobserved for the entire chromosome 3. There was significantvariation between backcross replicates for both bristle traits,indicating that additional loci affecting bristle number, linkedto Dl, were present in one backcross replicate but not the other.These linked loci had significant effects on variation in sexualdimorphism of abdominal bristle number. Terms involving variationbetween replicate vials were often significant in these andother analyses of the introgression lines, but these nongeneticterms will not be discussed further.

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Table 3. Variance components ( ${sigma}$ ²) and significance of mean squares (P) from analyses of variance of bristle number for Dl-H region introgression lines

Heterozygous effects, Dl-H region:
Each of the Sam Dl-H introgression lines was crossed to a straincontaining wild-type Dl and H alleles (Sam), a strain containinga mutant Dl allele (Dl³) and a strain containing a mutant Hallele; the variation in bristle number was determined amongthe three sets of heterozygous genotypes.

The results of analysis of variance of heterozygous bristlenumber are given in Table 3. There was significant variationin abdominal bristle number among lines for Dl-H/Sam and Dl-H/Hheterozygotes, but no other significant source of genetic variation.However, for the Dl-H/Dl³ heterozygotes, all of the significantvariation in abdominal bristle number among lines was in theS x L component, and additionally there was variation in heterozygouseffects and sex dimorphism in heterozygous effects between backcrosslines. Given the large S x L interaction for the Dl-H/Dl³ heterozygotes,analyses of variance of abdominal bristle number of these lineswere done separately for males and females (data not shown).There was no significant variation among lines for males ( ${sigma}$ ²= 0.217, P > 0.05), but highly significant among-line variationfor females ( ${sigma}$ ² = 1.390, P < 0.001). There was significantvariation in sternopleural bristle number among lines for Dl-H/Dl³and Dl-H/H heterozygotes, but not for Dl-H/Sam heterozygotes.For all three heterozygous genotypes, there was significantvariation in heterozygous sternopleural bristle number effectsbetween backcross replicates.

The average degree of dominance, k, of alleles affecting bristlenumber in the Dl-H region can be estimated from the regression,b, of line means of heterozygous bristle number on homozygousbristle number, as k = 2(b - 0.5) (MACKAY 1987 ). The rangeof k is from -1 (naturally occurring alleles completely recessive)through 0 (additive gene action) to +1 (naturally occurringalleles completely dominant). The regressions (b ± SE)of heterozygous abdominal bristle number on homozygous abdominalbristle number were 0.348 ± 0.038, 0.522 ± 0.075and 0.191 ± 0.046 for the Dl-H/Sam, Dl-H/Dl³ and Dl-H/Hheterozygous genotypes, respectively, giving respective estimatesfor k of -0.30 (partly recessive), 0.04 (additive) and -0.62(partly recessive). The regressions of heterozygous sternopleuralbristle number on homozygous sternopleural bristle number were0.334 ± 0.046, 0.681 ± 0.061 and 0.258 ±0.121, yielding estimates for k of -0.34 (partly recessive),0.36 (partly dominant) and -0.48 (partly recessive) for theDl-H/Sam, Dl-H/Dl³ and Dl-H/H genotypes, respectively.

These estimates of average degree of dominance are unbiasedonly if there is no error in estimating homozygous effects andthe degrees of dominance of alleles are uncorrelated with theirhomozygous effects (CABALLERO et al. 1997 ). The "reliabilityratio," V_L/(V_L + V_U), where V_L is the variance among lines andV_U is the error in estimating homozygous effects, is the amountby which an estimate of b from regression of heterozygous onhomozygous effects is biased toward zero (CABALLERO et al. 1997). For our data, the reliability ratios, estimated from variancecomponents in Table 3, are quite high (0.95 for abdominal bristlenumber and 0.93 for sternopleural bristle number) because homozygousline means are each estimated for 80 individuals. Thus, thereis little bias in estimates of degrees of dominance from errorin estimating homozygous effects. Further, nonlinear (quadratic)regression terms were not significant (data not shown), suggestingthat degrees of dominance of naturally occurring alleles affectingbristle number in the Dl-H gene region are not significantlycorrelated with their homozygous effects.

Quantitative complementation effects:
To detect whether naturally occurring alleles in the Dl-H generegion quantitatively fail to complement major morphologicalmutant alleles at Dl and H, we determined if there was significantvariation in the difference of line means of the Dl-H/Dl³ orDl-H/H heterozygotes (the Tester cross) and the Dl-H/Sam heterozygotes(the Control cross). Variation in Tester-Control effects (failureto complement) will occur if there is a difference in the degreeof dominance of the naturally occurring alleles against thewild-type and mutant standards.

The results of analyses of variance of heterozygous bristlenumber of the Dl-H region introgression lines, which includethe additional cross-classified fixed effect of Cross (C), aregiven in Table 4. The important new terms in these analysesare the main effect of C and the C x S, C x L and C x S x Linteraction terms. The main effect of C tests for a mean differencein bristle number between Dl or H and Sam heterozygotes, averagedover all lines and both sexes. The term was highly significantfor both bristle number traits in crosses of the introgressionlines to Dl and H, indicating the Dl and H alleles had largeheterozygous effects on bristle number. The C x S interactionterm tests for an effect of Dl or H on the sex dimorphism ofbristle number, averaged over all lines. Both candidate locusmutations strongly affected sex dimorphism of abdominal andsternopleural bristle numbers.

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Table 4. Variance components ( ${sigma}$ ²) and significance of mean squares (P) from analyses of variance of abdominal (AB) and sternopleural (ST) bristle number from quantitative complementation tests of Dl-H region introgression lines

The C x L and C x S x L interaction terms test for quantitativefailure to complement. The C x L term tests whether there isvariation in the difference in bristle number between the Testerand Control heterozygous genotypes of the different introgressionlines, averaged over both sexes. The C x S x L interaction testsfor variation in sex dimorphism of the failure to complement,that is, whether the C x L effects are different in males andfemales. We observed significant quantitative failure of theintrogression lines to complement abdominal and sternopleuralbristle effects of the Dl and H alleles. The failure of naturallyoccurring alleles in the Dl-H gene region to complement theabdominal bristle effect of Dl is complicated. There is complementationwhen Tester-Control scores are averaged over males and females(the C x L term is not significant), but highly significantvariation in failure to complement between males and females(the C x S x L interaction is highly significant). Analysesof variance of each sex separately (data not shown) reveal thatfailure to complement is observed only in females. The variancecomponent ( ${sigma}$ ²) for the C x L term in females was ${sigma}$ ² = 0.352 (0.001< P < 0.01), compared to ${sigma}$ ² = 0.003 (P > 0.05) in males.This is consistent with the observation above that there isvariation among Dl-H/Dl³ heterozygous lines for females only.The failure of naturally occurring alleles in the Dl-H regionto complement the sternopleural bristle effect of Dl, and theabdominal and sternopleural bristle effects of H, do not showthis sex specificity. The magnitude of the failure to complementcan be inferred from the C x L and C x S x L variance components.For abdominal bristle number, the sum of the C x L and C x Sx L effects is much larger for the Dl than the H tester allele,whereas the opposite is true for sternopleural bristle number;the C x L effect is much larger for the H than for the Dl testerallele, and C x S x L effects are not significantly differentfrom zero. This is consistent with the effects of the Dl andH mutants on bristle number; abdominal bristle number is increasedin Dl mutants, and sternopleural bristle number is decreasedin H mutants. Variation among line means in Tester - Control(T - C) effects in crosses to Dl³ and H is shown in Figure2.

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Figure 2. —Distributions of mean abdominal and sternopleural bristle number complementation effects (T-C) between heterozygous Dl-H/Dl³ or Dl-H/H(T) and heterozygous Dl-H/Sam (C) introgression lines. Solid bars are for male, and open bars for female complementation effects.

Correlations of line means between genotypes:
The correlations of line means for abdominal and sternopleuralbristle numbers across the different genotypes are given in Table 5. The whole chromosome 3 line means are not highly correlatedwith those of homozygous backcross lines for either bristletrait, as expected if other chromosome 3 loci than those inthe Dl-H gene region contribute to variation in bristle number.Neither are the chromosome 3 sternopleural and abdominal bristlenumber line means highly correlated with the Dl-H backcrossheterozygotes, for the above reason plus the expected reductionin heterozygous effect compared to homozygous effect for locithat are not dominant or overdominant. The correlations betweenhomozygous backcross bristle numbers and the Dl-H/Sam, Dl-H/Dl³and Dl-H/H heterozygotes are as expected from the regressionsof heterozygous on homozygous bristle numbers (see above). Thecorrelations of bristle numbers between the various heterozygousgenotypes are not high, reflecting the variable degrees of dominanceof the wild alleles in the mutant allele and Sam background.The Dl³ complementation effect was highly correlated with Dl-H/Dl³heterozygous effects, but not Dl-H/Sam heterozygous effects,for both bristle traits, presumably because the bristle numberalleles in the Dl-H region were more additive/dominant in theDl³ than in the Sam background. The H complementation effectwas positively correlated with Dl-H/H abdominal and sternopleuralbristle numbers, but negatively or not at all with the othergenotypes. Thus, positive correlations of the T - C H effectswith the Dl-H/H bristle numbers mean that the complementationeffect is smaller (less negative) in lines with high bristlenumbers and larger (more negative) in lines with lower bristlenumbers. Conversely, the negative association of the T - C Heffects in the other genotypes implies a reversal such thatlarge negative T - C effects are associated with high bristlenumbers, and vice versa, which could be a scale effect. Finally,correlations of mean T - C Dl³ abdominal bristle numbers withother genotypes were larger for females than males (Dl-H/Dl³)or only significant for females (C3, Dl-H, Dl-H/Sam and Dl-H/H)(data not shown), consistent with the observed female-specificcomplementation effect.

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Table 5. Correlations of line means across genotypes

Correlations between males and females:
The departure of the genetic correlation (r_G) in bristle numberbetween the sexes from unity indicates whether naturally occurringalleles affecting bristle number have sex-specific effects,that is, whether the genes are expressed and/or have the sameeffects in males and females. Across-sex genetic correlationsare significantly different from one when the S x L interactionterms in the analyses of variance (Table 2 Table 3 Table 4)are significantly different from zero. The S x L variance componentis significant for abdominal bristle number for the whole chromosome3, Dl-H homozygote and Dl-H/Dl³ heterozygote data, where itis, respectively, 29, 42, and 193% times the among-line variancecomponents. The genetic correlation of abdominal bristle numberbetween the sexes was computed for these data from variancecomponents as (ROBERTSON 1959 ), where the subscripts P, Mand F refer to the among-line variance components for the sexespooled and to male and female analyses, respectively (the separatesex analyses are not shown). The estimates were 0.811, 0.763and 0.499 for the whole chromosome 3, Dl-H homozygote and Dl-H/Dl³heterozygote genotypes, respectively. Further, the quantitativecomplementation test to Dl³ revealed highly significant C xS x L interaction variance, indicating sex-specific complementationeffects. The genetic correlation between the sexes for the differencein mean abdominal bristle number between the Tester and Controlcross (the complementation effect) was computed from variancecomponents as ^1/2 ; the point estimate is 0.304. The geneticcorrelation between male and female abdominal bristle numberin different genetic backgrounds is depicted graphically in Figure 3 as reaction norms; increasing departures of the geneticcorrelation from unity is manifested as more crossing of reactionnorms.

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Figure 3. —Norms of reaction for abdominal bristle number between males and females in genotypes with significant sex x line interaction variance.

For sternopleural bristle number, the S x L interaction termwas significant only for the whole chromosome 3 data, and themagnitude of the variance component was small, only 2% as largeas the among-line variance. Consequently, the genetic correlationof sternopleural bristle number between males and females forthis genotype, although significantly different from one, wasvery high (r_G = 0.984). Genetic correlations of sternopleuralbristle number between the sexes were not significantly differentfrom one in the other genetic backgrounds.

Correlations between bristle traits:
The correlations between line means for abdominal and sternopleuralbristle numbers are significantly different for the whole chromosome3 and the Dl-H region homozygotes. The correlation between bristletraits is not significantly different from zero for the aggregateof chromosome 3 loci (r = 0.180, averaged over males and females;P > 0.05). However, the traits are moderately, but significantly,positively correlated when only loci in the Dl-H region areconsidered (r = 0.431, averaged over sexes; P < 0.001). Thissuggests that pleiotropic effects of naturally occurring allelesaffecting bristle number are variable across bristle numberQTLs, and that alleles at other chromosome 3 bristle numberQTLs have negatively correlated effects on the two bristle traitsto compensate for the positive correlation in the Dl-H generegion. The correlations between bristle traits for the heterozygousgenotypes are not given because they are confounded with degreeof dominance, in the sense that they are increasingly similarto the homozygous Dl-H region correlations as the degree ofdominance of the wild-type alleles approaches k = 1 (completelydominant) and are, conversely, increasingly similar to the correlationsbetween these traits in the Sam, Dl³ and H background as thedegree of dominance of the wild-type alleles approaches k =-1(completely recessive).

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Loci in the Drosophila PNS development pathway are, a priori,candidate QTLs at which naturally occurring allelic variationcould cause quantitative genetic variation in numbers of adultsensory bristles (MACKAY 1985 ). Various disparate pieces ofexperimental evidence have specifically implicated the neurogenicloci Dl and H as Drosophila bristle number QTLs. In ascendingorder of credulity, the evidence is as follows. (1) The earliestefforts to analyze factors affecting long-term selection responsefor bristle number found, surprisingly, that the long-term selectionlines contained high frequencies of third chromosome recessivelethals with large heterozygous effects on bristle number, inthe direction of selection (e.g., CLAYTON and ROBERTSON 1957; FRANKHAM et al. 1968 ; YOO 1980B ). Mutations at Dl andH are generally recessive lethal with large heterozygous effectson bristle number (LINDSLEY and ZIMM 1992 ), but the lethalmutations in the long-term selection lines were never mappedbelow the level of chromosome [although YOO 1980B noted thattwo allelic lethals had a Dl-like wing vein phenotype]. (2)Fine-scale mapping of factors affecting response to divergentartificial selection for abdominal bristle number, from a basepopulation recently collected from nature, revealed a QTL witha large effect on abdominal and sternopleural bristle numbersin a 9-cM interval containing Dl and H (LONG et al. 1995 ).(3) Mutations at Dl and H interact genetically with high andlow bristle number selection lines containing naturally segregating(LONG et al. 1996 ) or spontaneous mutation (MACKAY and FRY1996 ) alleles at bristle number QTLs. Here, we provide furtherevidence supporting Dl and H as genetic loci at which naturallysegregating alleles affect quantitative variation in bristlenumber: QTLs in the Dl-H gene region both contribute to quantitativevariation in bristle number and fail to complement Dl and Hmutant alleles.

To test whether naturally occurring variation affecting bristlenumber is attributable in part to QTLs in the Dl-H gene region,we sampled isogenic third chromosomes from the same naturalpopulation used as the base for the selection-based QTL mappingexperiment of LONG et al. 1995 and substituted each into thestandard Sam inbred strain chromosome 1 and 2 background. Then,from each whole chromosome 3 line, we derived two lines in whichthe wild-type Dl-H region chromosomal segment was independentlyintrogressed into the Sam chromosome 3 background by 10 generationsof backcrossing. After 10 backcross generations, the Dl locus,and a linked chromosomal fragment originating from the wild-derivedthird chromosome of ~10 cM on either side of Dl, are expectedto remain in the otherwise Sam background (CROW and KIMURA 1970). The null hypothesis that variation among third chromosomesfor bristle number is not attributable in part to variationat loci in the 20-cM interval containing Dl and H is testedby the significance of the among-line component of variationfrom analysis of variance of bristle number of the introgressionlines. For both bristle traits, we reject this null hypothesisand conclude there is significant genetic variation for bristlenumber in the Dl-H region.

The Drosophila third chromosome is 110 map units long (LINDSLEYand ZIMM 1992 ); therefore, on average the introgressed wild-derivedfragments represent 18% of the chromosome. One extreme alternativehypothesis is the infinitesimal model, which assumes the underlyinggenetic basis for quantitative traits is a large number of QTLswith small allelic effects, evenly distributed over the chromosomes.Under this hypothesis, the prediction is that 18% of the wholechromosome 3 genetic variance for bristle number should be containedin the Dl-H introgressions. For abdominal bristle number, theamong-line and sex x line variance of the introgressions are,respectively, 36 and 53% that of the whole chromosome 3 variances—muchgreater than the infinitesimal model prediction. For sternopleuralbristle number, the among-line variance of the introgressionsis 8.3% of the whole chromosome 3 variance—less than theinfinitesimal expectation. These observations are consistentwith previous studies that showed that segregating (BREESE andMATHER 1957 ; SHRIMPTON and ROBERTSON 1988A , SHRIMPTON andROBERTSON 1988B ) and mutational (MACKAY et al. 1992A ; LYMANet al. 1996 ) variation for bristle number follows a leptokurticdistribution, with most of the variance attributable to a fewloci with large allelic effects and the remainder due to a largernumber of loci with smaller effects (ROBERTSON 1967 ).

The extent to which genetic variation for bristle number inthe Dl-H introgression lines could be attributable to geneticvariation at Dl and H was tested by crossing each introgressionline to Sam, the standard inbred line with wild-type Dl andH alleles (the Control cross) and to lines derived from Sam,into which mutations at Dl and H had been introgressed by 20generations of backcrossing (the Tester cross). The test forgenetic interaction of naturally occurring alleles affectingbristle number in the Dl-H region with the mutant Dl and H allelesis whether there is variation among the introgression linesin the difference of means between Tester and Control heterozygotes.The null hypothesis of no interaction was rejected for bothbristle traits at both candidate loci. However, the magnitudeof the complementation effects varied. For abdominal bristlenumber, the Dl complementation effect variance component was2.9x greater than the H complementation effect variance; whereasfor sternopleural bristle number, the H complementation effectvariance was 3.3x greater than the Dl complementation effectvariance. Further, the Dl complementation effect variance wassignificant only for females.

There are at least four possible genetic interpretations ofthe quantitative complementation test results. (1) Naturallyoccurring alleles at Dl have relatively large effects on femaleabdominal bristle number and smaller pleiotropic effects onsternopleural bristle number, in both sexes. Naturally occurringalleles at H have relatively large effects on sternopleuralbristle number and smaller pleiotropic effects on abdominalbristle number, in both sexes. (2) Naturally occurring allelesat Dl affect female abdominal bristle number and naturally occurringalleles at H affect sternopleural bristle number in both sexes.The abdominal bristle complementation effects at H and the sternopleuralbristle complementation effects at Dl are due, respectively,to epistatic interactions of the wild Dl abdominal bristle alleleswith the H mutation and the wild H sternopleural bristle alleleswith the Dl mutation. (3) There is naturally occurring allelicvariation affecting both abdominal and sternopleural bristlenumbers at either Dl or H, and the significant complementationeffect variance at the other locus is caused by epistatic interactionsof the mutation at this locus with the wild alleles. (4) Naturallyoccurring alleles affecting bristle number in the Dl-H region,but not at Dl nor H, interact epistatically with the mutantDl and H alleles. It is not possible to discriminate among thevarious allelism and epistasis hypotheses based on complementationtest results alone; all four interpretations are plausible.However, it becomes increasingly likely that one of hypotheses(1)–(3) is correct, as the size of the region containingthe candidate loci and putative additional interacting locishrinks. The combined evidence from mapping factors causingresponse to divergent artificial selection to the Dl-H interval(LONG et al. 1995 ), demonstrating appreciable segregating geneticvariation in the region (this article), and failure of selectedthird chromosomes (LONG et al. 1996 ) and Dl-H introgressionlines (this article) to complement mutant Dl and H alleles,strongly motivates a more fine-scale evaluation of the associationbetween molecular polymorphism at the candidate loci and phenotypicvariation in bristle number (LONG et al. 1998 ).

Our long-term goal is to understand the genetics and evolutionof quantitative traits in terms of complex genetics rather thancomplex statistics. To do this, it is necessary to know thegenetic loci contributing to mutational and segregating variationof the trait, and the additive, dominance, pleiotropic and epistaticeffects of spontaneous mutant and naturally segregating alleles,gene frequencies and per locus mutation rates (ROBERTSON 1967; BARTON and TURELLI 1989 ). This is a tall order, even forthe model system of Drosophila bristle number. The task wouldbe considerably simplified if the leading loci causing mostof the variation for the trait had similar genetic properties;one could then concentrate on evaluating the necessary parametersfor a representative few. How likely is this to be the case?Or, what is the variation among loci in additive, dominance,pleiotropic and epistatic effects? Unfortunately, the analysesof homozygous, heterozygous and pleiotropic effects of bristlenumbers in whole third chromosomes and Dl-H introgression lineshint at an underlying complexity and variation of allelic effectsbetween loci.

Consider first the average degree of dominance of segregatingalleles. This is an important parameter because the contributionto genetic variance of segregating alleles depends on theirdegree of dominance, as well as additive effects and gene frequency(FALCONER and MACKAY 1996 ). Naturally occurring variation forbristle number has been shown to be largely additive, with nosignificant directional dominance (CLAYTON et al. 1957 ; KIDWELLand KIDWELL 1966 ). However, we have observed that the degreeof dominance for bristle number of naturally occurring allelesin the Dl-H gene region varies significantly depending on theallele used as a standard. Average degrees of dominance forboth bristle traits range from additive or partly dominant relativeto Dl³ and partly recessive relative to H and Sam wild-typealleles. That the degree of dominance is not a fixed propertyof an allele, but must be considered relative to other alleles,is well known for mutant alleles of large effect, and will needto be taken explicitly into account when predicting the magnitudeof variation contributed by segregating alleles at genetic lociaffecting quantitative traits. The strong possibility that somefraction of naturally occurring variation for bristle numberis due to variation at candidate neurogenic loci raises theissue of variation in degrees of dominance across loci. Mutationsof large effect at known bristle loci are rarely strictly additiveand tend to be partly recessive or dominant. Furthermore, theaverage degree of dominance of mutations at bristle loci variesamong loci, with, for example, most achaete-scute mutationsrecessive and most Dl mutations dominant (LINDSLEY and ZIMM1992 ). It is possible that the observation of additive bristlenumber effects is an artefact of averaging over loci whose individualdominance deviations are predominantly dominant or recessive.

Phenotypic and genetic correlations between traits estimatedfrom response to selection and resemblance among relatives arealso averaged over all loci. The change in the correlation ofline means for homozygous abdominal and sternopleural bristlenumbers between the whole third chromosome, where the bristletraits were not significantly correlated, and the Dl-H regionhomozygotes, where the two traits were significantly positivelycorrelated, illustrates the important principle that an overalllack of correlation does not mean lack of pleiotropy. Rather,there appears to be variation in pleiotropic effects for abdominaland sternopleural bristle numbers among the third chromosomeloci contributing to variation for these traits, as the positivecorrelation observed for the Dl-H gene region must be balancedby negative (or no) pleiotropic effects at other loci to reducethe net correlation of traits on the whole chromosome 3. Thisis also true for the genetic correlation of abdominal bristlenumber between males and females. Over 50% of the whole chromosome3 sex x line variance is accounted for by loci in the Dl-H generegion, which implies that, for at least some chromosome 3 locioutside this region, the genetic correlation between the sexesfor abdominal bristle number must be higher. Variation in pleiotropiceffects between loci is, however, a common feature of mutationsat candidate bristle loci: mutations at Dl tend to increaseand mutations at H tend to decrease both abdominal and sternopleuralbristle numbers, whereas mutations at scabrous, a chromosome2 candidate bristle locus (LAI et al. 1994 ), decrease sternopleuralbristle number in both sexes and increase abdominal bristlenumber in females only (T. F. C. MACKAY, unpublished results).

An unusual and recently observed feature of segregating (MACKAYand LANGLEY 1990 ; LONG et al. 1995 , LONG et al. 1998 ; thisreport) and mutational (MACKAY et al. 1992A , MACKAY et al.1992B , MACKAY et al. 1994 , MACKAY et al. 1995 ; LOPEZ andLOPEZ-FANJUL 1993 ; LYMAN et al. 1996 ; MACKAY and FRY 1996) quantitative genetic variation for abdominal, and to a lesserextent, sternopleural, bristle numbers is that homozygous, heterozygousand epistatic effects are often highly sex specific. Althoughlarge sex-specific abdominal bristle effects had been reportedpreviously in long-term selection lines (CLAYTON and ROBERTSON1957 ; FRANKHAM 1968 ; FRANKHAM et al. 1978 ; FRANKHAM 1980), they were shown to be caused by mutations at the bobbed locus,which is duplicated on the X and Y chromosomes, and thus thesex-specific effects were not thought to be general. However,sex-specific QTL effects have been observed for Drosophila olfactorybehavior (ANHOLT et al. 1996 ; MACKAY et al. 1996 ) and longevity(MAYNARD SMITH 1959 ; NUZHDIN et al. 1997 ) and may be a commonproperty of quantitative variation in this and other species.Past inferences from experimental results for Drosophila bristlenumber have been accurate predictors of the properties of quantitativegenetic variation for equivalent traits in other species (FRANKHAM1989 ). The general pattern of variation in sex dimorphism observedis that variation among the same set of genotypes is much greaterfor females than males, perhaps reflecting stronger geneticcanalization in males than females. Sex-specific QTL effectsare a special case of genotype x environment interaction, wherethe sexes are the different environments, and could in somecircumstances contribute to the maintenance of quantitativegenetic variation (GILLESPIE and TURELLI 1989 ). A low geneticcorrelation between the sexes also facilitates the evolutionof further sexual dimorphism (LANDE 1980 , LANDE 1981 ). Furtherfine-scale mapping of the large, female-specific, Dl³ abdominalbristle number complementation effect should prove particularlyinteresting.

ACKNOWLEDGMENTS

We thank FAYE LAWRENCE and LUCY REID for excellent and dedicatedtechnical assistance, and TONY LONG for comments on the manuscript.This work was supported by grants GM-45344 and GM-45146 fromthe National Institutes of Health.

Manuscript received August 29, 1997; Accepted for publication February 27, 1998.

LITERATURE CITED

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

ANHOLT, R. R. H., R. F. LYMAN, and T. F. C. MACKAY, 1996 Effects of single P element insertions on olfactory behavior in Drosophila melanogaster. Genetics 143:293-301[Abstract].

ARTAVANIS-TSAKONAS, S., K. MATSUNO, and M. E. FORTINI, 1995 Notch signaling. Science 268:225-232[Abstract/Free Full Text].

BARTON, N. and M. TURELLI, 1989 Evolutionary quantitative genetics: how little do we know? Annu. Rev. Genet. 23:337-370