Identification of X-Linked Genes Required for Migration and Programmed Cell Death of Drosophila melanogaster Germ Cells

Identification of X-Linked Genes Required for Migration and Programmed Cell Death of Drosophila melanogaster Germ Cells

Clark R. Coffman^a, Rachel C. Strohm^a, Fredrick D. Oakley^a, Yukiko Yamada^a, Danielle Przychodzin^b, and Robert E. Boswell^b
^a Department of Zoology and Genetics, Iowa State University, Ames, Iowa 50011-3260
^b Department of Molecular, Cellular and Developmental Biology, University of Colorado, Boulder, Colorado 80309

Corresponding author: Clark R. Coffman, 3258 Molecular Biology Bldg., Iowa State University, Ames, IA 50011-3260., ccoffman{at}iastate.edu (E-mail)

Communicating editor: T. SCHÜPBACH

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Drosophila germ cells form at the posterior pole of the embryoand migrate to the somatic gonad. Approximately 50% of the germcells that form reach their target. The errant cells withinthe embryo undergo developmentally regulated cell death. Priorstudies have identified some autosomal genes that regulate germcell migration, but the genes that control germ cell death arenot known. To identify X-linked genes required for germ cellmigration and/or death, we performed a screen for mutationsthat disrupt these processes. Here we report the identificationof scattershot and outsiders, two genes that regulate the programmeddeath of germ cells. The scattershot gene is defined by a mutationthat disrupts both germ cell migration and the death of germcells ectopic to the gonad. Maternal and zygotic expressionof scattershot is required, but the migration and cell deathfunctions can be genetically uncoupled. Zygotic expression ofwild-type scattershot rescues germ cell pathfinding, but doesnot restore the programmed death of errant cells. The outsidersgene is required zygotically. In outsiders mutant embryos, theappropriate number of germ cells is incorporated into the gonad,but germ cells ectopic to the gonad persist.

CELL migration and programmed cell death play critical rolesin animal development, immune system function, wound healing,angiogenesis, and metastasis (LAUFFENBURGER and HORWITZ 1996; JACOBSON et al. 1997 ; HOLDER and KLEIN 1999 ; MEIER etal. 2000 ). Many cells are formed in one part of the body andmust migrate to their ultimate locations to function. A commonstrategy is to overproduce cells and then eliminate those thatare no longer needed or that are potentially dangerous to theanimal. The control of cell movements and cell death in an organismmust be precisely regulated, and these processes require theintegration of a wide range of signals between and within cells.

The germ cells of Drosophila provide an excellent system forthe study of cell migration and cell death. The movements ofthe germ cells have been well documented, and the eliminationof ectopic and/or supernumerary germ cells occurs with greatefficiency (SONNENBLICK 1941 , SONNENBLICK 1950 ; COUNCE 1963; FULLILOVE and JACOBSON 1978 ; UNDERWOOD et al. 1980 ; TECHNAUand CAMPOS-ORTEGA 1986 ; HAY et al. 1988 ; LASKO and ASHBURNER1990 ; SMITH et al. 1992 ; JAGLARZ and HOWARD 1994 , JAGLARZand HOWARD 1995 ; WARRIOR 1994 ; WILLIAMSON and LEHMANN 1996; CAMPOS-ORTEGA and HARTENSTEIN 1997 ; MOORE et al. 1998 ; WYLIE 1999 , WYLIE 2000 ; STARZ-GAIANO and LEHMANN 2001 ).Selected features of germ cell movements and the eliminationof germ cells ectopic to the gonad are shown in Fig 1. Priorstudies have shown that $~$ 50% of the primordial germ cells thatform successfully complete migration and are incorporated intothe somatic gonad (SONNENBLICK 1950 ; UNDERWOOD et al. 1980; TECHNAU and CAMPOS-ORTEGA 1986 ). Primordial germ cells thathave been labeled using horseradish peroxidase or radioactivethymidine do not transdifferentiate, and very few transplantedcells persist outside of the gonads (UNDERWOOD et al. 1980 ; TECHNAU and CAMPOS-ORTEGA 1986 ). Collectively, these studiesdemonstrate that germ cells ectopic to the gonad die and thata mechanism regulating germ cell survival must exist withinthe embryo.

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Figure 1. Dynamics of germ cell development. Some of the stages of germ cell development are shown. The germ cells are labeled utilizing a fat facets-lacZ reporter transgene. Anterior is to the left in all panels. (A, B, and D) Lateral views. (C, E, F, and G) Dorsal views. (A) Germ cells form at the posterior pole of the embryo. (B and C) Germ band extension is complete and the germ cells are contained within the posterior midgut epithelium. (D and E) Germ cell migration through the posterior midgut epithelium is almost complete, and the germ cells are separating laterally into two populations. (F) Germ cells have migrated to and are coalescing with the somatic gonad precursor cells in a germ band retracted embryo. (G) Germ cell migration is complete. Note the absence of labeled cells outside of the gonads.

To date, no X-linked genes with roles in germ cell migrationor programmed cell death have been reported. Screens of thesecond and third chromosomes identified some genes necessaryfor germ cell migration in Drosophila, but their roles remainenigmatic (KOBAYASHI et al. 1996 ; ZHANG et al. 1996 ; BOYLEet al. 1997 ; ZHANG et al. 1997 ; ASAOKA et al. 1998 ; BROIHIERet al. 1998 ; FORBES and LEHMANN 1998 ; MOORE et al. 1998; VAN DOREN et al. 1998 ; DESHPANDE et al. 1999 , DESHPANDEet al. 2001 ; STARZ-GAIANO et al. 2001 ). Our understandingof the regulation of germ cell development is far from complete,as this process must involve the functions of additional genes.Therefore, we conducted a screen of the X chromosome for genesthat are required for normal germ cell development. When mutated,all of the genes identified in our screen altered the distributionof germ cells in the early Drosophila embryo. These mutationsare informative to the study of germ cell migration and/or celldeath, as they do not map to loci with previously describedroles in these processes.

We report the identification and initial characterization oftwo genes. The first, scattershot (sctt), is maternally andzygotically required. This gene, when mutated, severely disruptsboth germ cell migration and developmental cell death. In embryosfrom sctt/sctt mutant mothers, very few of the germ cells successfullymigrate to the gonad. In addition, those germ cells ectopicto the gonad retain germ cell characteristics. Although thegerm cell migration in sctt mutants is severely altered, germcell formation, somatic gonad development, and body patternappear normal. Homozygous female and hemizygous male sctt mutantembryos are viable and fertile, although fertility is greatlyreduced. The sctt gene is only the third gene identified inDrosophila with a demonstrated role in germ cell migration whoseproduct is maternally contributed. The other two are polar granulecomponent (pgc) and nanos (nos; KOBAYASHI et al. 1996 ; NAKAMURAet al. 1996 ; ASAOKA et al. 1998 ; FORBES and LEHMANN 1998; DESHPANDE et al. 1999 ). Interestingly, zygotic expressionof a wild-type copy of sctt rescues the germ cell migrationdefect, but fails to rescue the programmed cell death phenotypeof sctt mutant embryos. A second gene, outsiders (out), mustbe expressed zygotically and has a function in the death ofgerm cells that fail to reach the gonad. The number of germcells that reach the gonad is the same in out/out embryos andin unmutagenized controls. However, many additional cells outsideof the gonad continue to express germ cell markers. Thus, bothsctt and out are necessary for the execution of a cell deathprogram, and sctt has an additional role in germ cell pathfinding.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Mutagenesis and screening:
To isolate X-linked mutations affecting germ cell development,3475 independent mutagenized lines were screened. A P[w⁺, fatfacets-lacZ] transgene that is expressed specifically in thegerm cells of the embryo was used to determine the locationof the germ cells (FISCHER-VIZE et al. 1992 ). The screen isdiagrammed in Fig 2. Three- to 4-day-old w¹¹¹⁸, P[w⁺, fat facets-lacZ]/Ymales were mutagenized using 25 mM ethyl methane sulfonate (EMS)in 1% sucrose (LEWIS and BACHER 1968 ) and crossed to y w hnt¹¹⁴²,P[ry⁺, FRT¹⁰¹]/FM7, Df(1)KA14/FM7c, or Df(1)HA32/FM7c, P[ry^+t7.2,ftz-lacZ] (FM7Z) virgin females. After 4 days, the adults werecleared from the bottles. The resulting female offspring carryingthe balancer chromosome were then individually crossed to FM7/Y,FM7c/Y, or FM7Z/Y males to establish stocks. The stocks werethen expanded, and the embryos were collected using 50-ml conicaltubes with apple juice-agar medium in the caps. Chorion removal,fixation, and staining were carried out in 48-well custom stainingtrays. The germ cells were labeled using X-Gal as the substrate(SIMON et al. 1985 ; HOLMES et al. 1998 ).

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Figure 2. Diagram of a screen for X-linked mutations affecting germ cell development. Males were mutagenized using EMS. The mutagenized X chromosome (*) was isolated over an FM7 balancer chromosome. Depending upon the viability and fertility of the mutagenized X chromosome, either homozygous or balanced stocks were established. Overnight collections of embryos from these stocks were used for staining.

The nonmutagenized w¹¹¹⁸, P[w⁺, fat facets-lacZ] parental stockhad a very low percentage of embryos with any germ cells outsidethe gonad. During the screen and subsequent analyses, embryoswere scored as mutant if they had four or more germ cells ectopicto the gonad. For brevity, the parental w¹¹¹⁸, P[w⁺, fat facets-lacZ],mutagenized w¹¹¹⁸ sctt, P[w⁺, fat facets-lacZ], and w¹¹¹⁸ out,P[w⁺, fat facets-lacZ], chromosomes will be referred to as faf-lacZ,sctt, and out, respectively.

Mapping and complementation analyses:
To determine the location of the sctt and out mutations, themutant lines were tested for complementation using the X chromosomedeletion stocks available from the Bloomington and Umeåstock centers (FLYBASE 1999 ). Since sctt is required maternally,sctt/Df(1) females were generated and their offspring were testedfor abnormal germ cell development. The location of out wasestablished by crossing Df(1)/balancer virgin females to out/Ymales. The germ cell phenotype of the progeny of the Df(1)/outfemales was then assayed.

Recombination mapping to localize sctt was performed using thesctt mutant chromosome and w¹¹¹⁸ cv¹ wy⁷⁴ⁱ f¹, sc¹ ec¹ cv¹ wy⁷⁴ⁱf¹, or y¹ w¹ cv¹ ct⁶ v¹ marker chromosomes. The insertion siteof the P[w⁺, fat facets-lacZ] was determined to be 18F-19A byin situ hybridization of a digoxygenin-labeled white probe (akind gift from Joseph Heilig) to salivary gland chromosomes(O'HARE et al. 1984 ; JOHNSON-SCHLITZ and LIM 1987 ; TAUTZand PFEIFLE 1989 ; KLINGLER and GERGEN 1993 ). Virgin femaleshomozygous for the sctt mutant chromosome were crossed to malescarrying the marker X chromosome. Recombination occurred inthe F₁ females, which were crossed to FM7c/Y males. IndividualF₂ males from this cross that carried a recombinant chromosomewere then crossed to y w hnt¹¹⁴², P[ry⁺, FRT¹⁰¹]/FM7c, Df(1)KA14/FM7c,or Df(1)HA32/FM7Z virgin females. Each individual recombinantX chromosome was then isolated over a balancer chromosome toestablish a stock. The balancer chromosome was removed to yieldan independent homozygous recombinant line. Embryos collectedfrom F₅ or later mothers homozygous for the recombinant X chromosomewere scored for the sctt phenotype using X-Gal staining of 12-to 15-hr embryos.

Complementation tests between sctt, out, and the other linesobtained in the screen were also performed. To test for complementationof the maternal-effect germ cell migration phenotype of sctt,virgin females from the remaining lines were crossed to sctt/Ymales. The offspring from trans-heterozygous sctt/test chromosomeF₁ females were then assayed for complementation. The out complementationgroup was determined by testing out/FM7Z and/or out/out femalescrossed to males from the other lines, if the test line producedviable males. If the X chromosome carried a lethal mutation,heterozygous test chromosome/FM7Z virgin females were crossedto out/Y males. The germ cell phenotype of the progeny was thenassayed by ß-galactosidase (ß-Gal) staining.

Fertility assay and ovary dissections:
To test fertility, individual male and female offspring of sctt/sctt,sctt/FM7, or faf-lacZ/faf-lacZ females were crossed to Ore-Rflies and placed in vials for 5–7 days. For the crossestesting male fertility, vials were scored for the presence oflarvae or pupae. A vial that contained no offspring was scoredas sterile only if adults of both sexes were still alive inthe vial and unhatched eggs were present. In the crosses thattested female fertility, vials were scored for the presenceof eggs or offspring. In these cases, a vial that did not containeggs was scored as sterile only if the test female was stillalive at the end of the trial period.

Ovaries from some of the test females were dissected in PBST(137 mM NaCl, 2.7 mM KCl, 10 mM Na2HPO4, 1.8 mM KH2PO4, 0.3%Triton X-100, pH 7.2; SAMBROOK et al. 1989 ) to assay the statusof ovary development. Ovaries containing late-stage oocyteswere scored as normal (KING 1970 ; MAHOWALD and KAMBYSELLIS1980 ; SPRADLING 1993 ). Agametic ovaries had no detectableoocytes. Rudimentary ovaries contained early oogenic stages(younger than stage 9), but no late-stage oocytes. The datapresented include only those females from which both ovarieswere recovered in the dissection.

Germ cell counts:
To determine the number of ß-Gal-positive germ cellspresent in 11- to 12-hr faf-lacZ control, sctt, or out embryos,embryos were collected for 1 hr on apple juice caps and thenaged 11 hr at 25°. ß-Gal staining was performedas above and germ cells were counted using differential interferencecontrast microscopy. All of the cells counted were positivefor ß-Gal activity and exhibited the spherical nucleusand large cell size characteristic of germ cells at this stageof development (RABINOWITZ 1941 ; POULSON 1950 ; UNDERWOODet al. 1980 ). The gonadal sheath cells were used to determinethe boundary of the gonad. Statistical analyses were performedusing Minitab Statistical Software (Minitab, State College,PA) or JMP version 4.0 (SAS Institute, Cary, NC).

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Screen for mutants defective in germ cell development:
X-linked genes with functions required for germ cell developmentwere identified in an EMS mutagenesis screen of 3475 independentlines. Germ cells ectopic to the gonad were observed in 39 lines.Seventeen of these lines exhibited >40% penetrance and werekept for further analyses. In the four most severe mutants,the germ cells are scattered throughout the posterior half ofthe embryo and very few, if any, germ cells populate the gonad.This scattered germ cell phenotype is observed in two homozygousviable lines and two lines that are homozygous lethal. A secondclass of 13 lines exhibit less severe phenotypes that are characterizedby visible clusters of germ cells in the position of the gonadand four or more germ cells located outside of the gonads. Thisgroup consists of eight homozygous viable alleles and five chromosomeswith lethal mutations. Complementation analyses of these 17lines reveal that the mutations we isolated represent at leastfour complementation groups. Detailed analyses of the sctt andout genes are described here.

Genetic characterization of sctt:

A single recessive allele of sctt was isolated (Fig 3). Thisallele is highly penetrant (>94%), and disruption of the germcell staining pattern requires that the mother be homozygousmutant (Table 1). The offspring of sctt/sctt females will bereferred to as sctt mutant embryos unless otherwise specified.This allele is complemented by all of the X chromosome deletionstocks available from the Bloomington and Umeå stock centers,which represent $~$ 80% of the X chromosome. Since a noncomplementingdeletion was unavailable, we determined the genetic map positionby recombination mapping of sctt using marked X chromosomes.We analyzed 32 lines with a recombination event between cv andwy and 21 lines with a recombination event between y or sc andcv. These analyses place sctt within 1 map unit of cv. The cvgene maps to 1-13.7 on the genetic map and is predicted to liewithin polytene chromosome bands 5A13–5B1 (LINDSLEY andZIMM 1992 ; FLYBASE 1999 ). The Dp(1:Y)dx⁺5 chromosome carryingpolytene chromosome bands 4C11;6D8 zygotically rescues the scttgerm cell migration phenotype. This indicates that sctt is withinthe 4C11:6D8 interval. Three gaps in the deletion stocks fallwithin the region delimited by our recombination mapping. Itis likely that sctt is located in one of these regions not representedby the deletion stocks. It is formally possible that the scttphenotype is the result of two independent mutations. If thisis the case, they are very tightly linked. The sctt phenotypeis complemented by all P-element insertions and previously identifiedmutations tested to date.

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Figure 3. Mutation of sctt results in aberrant germ cell migration and retention of germ cell marker expression in germ cells outside of the gonad. Lateral views of (A) sctt mutant and (C) wild-type embryos showing germ cells migrating across the posterior midgut epithelium (arrows). Germ cell formation and migration are indistinguishable from a wild-type embryo. Dorsal views of stage 14 sctt (B) and wild-type (D) embryos are shown. Note that very few germ cells, if any, in the sctt embryo are located in the regions of the gonad (arrows). Also, many germ cells outside of the gonad continue to express Faf-ß-Gal. The embryos shown in A–D were stained in parallel. (E) An sctt mutant embryo double labeled for the 412 retrotransposon, a marker of somatic gonadal mesoderm, and for the Faf-ß-Gal germ cell marker. The somatic gonadal mesoderm (arrows, brown) shows a wild-type staining pattern. The germ cells are blue and are seen scattered throughout the posterior of the embryo.

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Table 1. The scattershot phenotype is maternal effect and highly penetrant

Genetic characterization of out:

The out complementation group consists of six recessive alleles(Table 2). In out mutants, clusters of Faf-ß-Gal-expressinggerm cells are clearly localized to each gonad, but germ cellsectopic to the gonad are also prominent (Fig 4). Three allelesare homozygous viable (out¹, out², and out³), and three allelesare homozygous lethal (out⁴, out⁵, and out⁶). The product ofthe out gene is required zygotically. Penetrance of the mutantphenotype ranges from 65.6% for out⁶ to 93.7% for out¹. Thethree viable alleles, out¹, out², and out³, fail to complementthe germ cell mutant phenotype of each other and, for each ofthese alleles, this phenotype is uncovered by Df(1)JA27, whichis reported to be a deletion of polytene chromosome bands 18A5;18D1(FLYBASE 1999 ). The three viable alleles fail to complementout⁴ and out⁵. Interestingly, out⁶ is not complemented by out¹and out³ but is complemented by out² (Table 2). Embryos fromthe three lethal lines appear to have normal segmentation; however,the out⁴ and out⁵ lines exhibit increased pupal lethality. Thephenotypes of Df(1)JA27/Y males and Df(1)JA27/out¹ hemizygousfemales are more severe than any combination of out allelesfrom our screen. The germ cell phenotype associated with theDf(1)JA27 chromosome is recessive, as Df(1)JA27/+ embryos havea wild-type germ cell staining pattern. The out phenotype iscomplemented by all P-element and known mutations within the18A5;18D1 interval that we have tested. We have not determinedwhether the lethality associated with out⁴, out⁵, and out⁶ isdue to the out mutation or is due to a second mutation presenton these chromosomes.

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Figure 4. The out mutants are deficient in the elimination of ectopic germ cells. (A) A dorsal view of a stage 14 out/out mutant embryo shows two gonads. However, many cells outside of the gonad continue to stain for Faf-ß-Gal. (B) Dorsal view of a wild-type embryo stained in parallel with the embryo shown in A.

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Table 2. The out complementation group consists of six recessive alleles

Mutation of sctt disrupts germ cell migration and developmentally regulated cell death:
In sctt mutant embryos, germ cell development, as visualizedby the Faf-ß-Gal marker, appears normal prior to migration.Germ cells form at the posterior pole, and they are incorporatedinto the posterior midgut (PMG) pocket at the completion ofgerm band extension (stage 10; CAMPOS-ORTEGA and HARTENSTEIN1997 ). The germ cells then transit the epithelium of the PMG(JAGLARZ and HOWARD 1994 , JAGLARZ and HOWARD 1995 ; WARRIOR1994 ; CALLAINI et al. 1995 ; Fig 3A). However, very few,if any, of the germ cells in sctt mutant embryos successfullymigrate to and become incorporated into the developing gonad.Instead, the germ cells disperse throughout the posterior halfof the embryo and continue to express the Faf-ß-Galmarker (compare Fig 3B and Fig D, and Fig 5A). This phenotypereveals that this sctt mutation disrupts two processes. First,cell migration is severely impaired. Second, the cells thatdo not reach the gonad fail to undergo cell death. Despite theseverity of the germ cell phenotype, homozygous sctt mutantsare viable, and these individuals do not display any detectablemorphological abnormalities as embryos or adults, with the exceptionof agametic gonads (see below).

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Figure 5. The sctt germ cell migration phenotype can be paternally rescued. Zygotic expression of a wild-type copy of sctt rescues the germ cell migration defect, but cells outside of the gonad continue to express germ cell markers. Two embryos from sctt/sctt mutant mothers are shown. (A) The phenotype observed in homozygous sctt/sctt or hemizygous sctt/Y individuals. (B) An sctt/+ embryo. Note the small clusters of germ cells that have successfully migrated to the gonad (arrows in B).

In the homozygous sctt stock, 97.8% of the embryos display theextremely severe phenotype shown in Fig 3B. In contrast, only3–4.5% of embryos from sctt/FM7 mothers and 6.5% of embryosfrom the unmutagenized faf-lacZ/faf-lacZ stock have four ormore labeled germ cells located outside of the gonad (Table 1).The germ cell migration defect is observed only among theoffspring of homozygous sctt mutant mothers, and it is not evidentin the sctt/sctt or sctt/Y offspring of sctt/FM7 females crossedto sctt/Y males. Therefore, the sctt mutation isolated in thisscreen is recessive and a maternal effect. Also, the phenotypesof sctt/sctt and sctt/Y embryos from sctt/sctt mutant mothersare equivalent.

The pathfinding and cell death defects in sctt embryos can begenetically uncoupled:

To better understand the relationship between germ cell migrationand programmed cell death, we performed additional genetic andphenotypic analyses of sctt mutant embryos. We reasoned thatif sctt function is required at different times for either germcell migration or the elimination of ectopic germ cells, thenwe might be able to separate differing temporal requirementsthrough paternal contribution of a wild-type copy of sctt. Ifsctt function were required both maternally and zygoticallyfor germ cell migration, then an embryo expressing a wild-typecopy of sctt would display a less severe germ cell migrationphenotype. Alternatively, if the cell death phenotype were rescuedby zygotic expression of a wild-type copy of sctt, then onlythose germ cells that successfully migrated to the gonad wouldcontinue to express Faf-ß-Gal, while those cells outsideof the gonad would undergo programmed cell death.

When sctt/sctt females are crossed to Ore-R males, the offspringof this cross fall into two phenotypic classes (Table 1, line2; Fig 5). The first class displays the severe germ cell migrationdefect seen in the homozygous sctt line, and the germ cellsoutside the gonad continue to express Faf-ß-Gal (Fig 5A).In these embryos, so few germ cells successfully migratethat the gonads cannot be easily identified in a ß-Gal-stainedembryo. This phenotype was observed in 60% (n = 653) of theembryos. In the remaining embryos, an increased number of germcells successfully migrate to the gonad, but many cells outsideof the gonad continue to express Faf-ß-Gal (Fig 5B).To test the hypothesis that the less severe phenotype is theresult of paternal rescue, we crossed sctt/sctt females to FM7Z/Ymales. This hypothesis predicts that the more severe phenotypewill be observed in sctt/Y embryos, while the less severe phenotypewill be observed in sctt/FM7Z embryos. The FM7Z chromosome carriesa wild-type sctt gene. The sctt/FM7Z female embryos resultingfrom this cross stain blue due to the presence of the ftz-lacZtransgene. The severe sctt phenotype was observed in 217/218sctt/Y embryos (Table 1, line 3). Among the lightly stainedsctt/FM7Z female embryos, ß-Gal-stained germ cellswithin the gonad as well as germ cells located outside of thegonad were observed. Therefore, zygotic expression of wild-typesctt from the paternal X chromosome improves germ cell migration.The recessive maternal effect, the recessive zygotic phenotypes,and the zygotic rescue data collectively suggest that this scttallele is loss of function.

We counted the number of germ cells that successfully migratedto the gonad in embryos that were born to sctt/sctt mothersbut received a wild-type paternal copy of sctt. Interestingly,the same numbers of germ cells were observed within the gonadsof control and paternally rescued embryos at 11–12 hrof development (Table 3). We counted an average of 13.7 germcells within the two gonads of faf-lacZ embryos (n = 50) and12.7 germ cells incorporated into the two gonads of sctt/+ rescuedembryos (n = 50). These values are not statistically different(P = 0.09, Student's t-test). The average of 6–7 germcells per gonad is within the range reported for other Drosophilalines (SONNENBLICK 1941 , SONNENBLICK 1950 ; UNDERWOOD etal. 1980 ; HAY et al. 1988 ). These data support the conclusionthat zygotic expression of a wild-type copy of sctt rescuesthe germ cell migration defect associated with sctt mutant embryos.However, an average of 7.7 germ cells was observed outside ofthe gonads in the rescued embryos. The range was 4–16germ cells ectopic to the gonad, and most of the Faf-ß-Galpositive cells retained a characteristic germ cell morphology(RABINOWITZ 1941 ; POULSON 1950 ; UNDERWOOD et al. 1980 ).Thus, the developmental cell death of ectopic germ cells isnot rescued by zygotic expression of wild-type sctt. The averagetotal number of germ cells observed is 17.7 (n = 50) in sctt/scttor sctt/Y embryos and 20.4 in sctt/+ embryos (n = 50; Table 3).Both of these means are significantly higher than the totalgerm cell number of 14.0 observed in controls (P $<=$ 0.0001, Student'st-test).

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Table 3. Germ cell numbers observed in out and sctt mutants

Fertility is greatly reduced in sctt mutants:
The sctt phenotype cosegregates with reduced fecundity. To quantitatethis phenotype, we performed fertility tests. Male and femaleoffspring of faf-lacZ/faf-lacZ control, sctt/FM7, and sctt/scttfemales were assayed for fertility. When individual test malesor females from faf-lacZ/ faf-lacZ or sctt/FM7 mothers werecrossed to Ore-R flies of the opposite sex, the fertility ratewas >90% (Table 4). However, sctt males from sctt/sctt mutantmothers were fertile in only 33.7% of the crosses (n = 285).When sctt/sctt females from sctt/sctt mutant mothers were matedto Ore-R males, 41.7% of the females produced offspring (n =163). The remaining females failed to lay any eggs. Interestingly,sctt/+ females from sctt/sctt mothers were as fertile as wild-typeanimals (100%, n = 135). Therefore, the zygotic rescue of thegerm-cell-migration defect associated with the sctt mutationrestores fertility to wild-type levels. This is consistent withthe observation that wild-type numbers of germ cells are incorporatedinto the gonad of these paternally rescued embryos. The ovariesfrom these individuals were also normal (see below).

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Table 4. Decreased fertility is associated with the sctt mutation

Agametic ovaries occur at a high frequency in sctt mutants:
The sterility associated with the sctt mutation suggested alack of germ-line stem cells within the gonad, an arrest ofoogenesis, or abnormal somatic gonad development. We investigatedthese possibilities by analyzing ovarian development in differentmutant backgrounds. An absence of germ-line stem cells or anearly disruption of oogenesis would result in agametic ovaries,while abnormal somatic gonad development would lead to a lackof or malformation of somatically derived ovarian structures.

The formation of a functional gonad requires the interactionof the germ cells with the somatic gonadal mesoderm. To testwhether the somatic gonad cell fate is specified in sctt mutantembryos, we used the 412 retrotransposon as a molecular markerfor somatic gonad differentiation. The 412 retrotransposon probelabels gonadal mesoderm cells even in the absence of germ cells(BROOKMAN 1992). The in situ hybridization staining patternin sctt mutant embryos is indistinguishable from wild type (Fig 3E).In addition, the fact that sctt embryos produce viableand fertile adults, albeit at a lower frequency, demonstratesthat the gonad can function if populated by germ cells.

The dissection of ovaries from control and sctt mutants revealsthat the sterility associated with the sctt mutation is theresult of a lack of germ-line stem cells or a very early arrestof oogenesis. Of the ovaries dissected from 87 offspring offaf-lacZ/faf-lacZ or sctt/FM7 females, 99% were normal (n =174 ovaries; Table 5; Fig 6B). Two ovaries from the sctt/FM7test lines were scored as rudimentary because they did not containoocytes older than stage 9 (KING 1970 ; SPRADLING 1993 ). Incontrast, among the sctt/sctt female offspring of sctt/scttmutant mothers, 57% of the ovaries were agametic, 11% were rudimentary,and 32% were normal (n = 122). An example of agametic ovariesfrom an sctt/sctt mutant is shown in Fig 6A. The gonadal defectscorrelate with fecundity. We dissected 32 females that did notlay eggs. Of these, 24 had two agametic ovaries, 6 had two rudimentaryovaries, and 2 had one agametic ovary and one rudimentary ovary.We examined an additional 29 sctt females that did lay eggs.All of these had at least one normal ovary and, in 10 of them,both ovaries appeared normal. Interestingly, 97% (n = 120) ofthe ovaries from sctt/+ females from sctt/sctt mothers werewild type. Therefore, zygotic rescue of the germ cell migrationdefect leads to nearly normal ovary formation and restorationof wild-type fertility levels.

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Figure 6. The sterility associated with the sctt mutation is due to an absence of germ cells within the gonad. (A) Agametic ovaries from an sctt mutant have a normal complement of somatic gonad-derived structures, but lack germ cells. (B) Wild-type ovaries. Both photographs are taken at the same magnification.

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Table 5. The sctt mutation causes a high percentage of agametic ovaries

The out mutation impairs cell death of errant germ cells:
An example of an out¹/out¹ mutant embryo is shown in Fig 4A.Somatic gonad development as assayed by the 412 retrotransposonis normal (data not shown). The out gene product is requiredzygotically, and the six out alleles result in many ß-Gal-labeledgerm cells outside of the gonad. These ß-Gal-positivecells can be seen outside of the gonad until at least 15 hrof development. At this time, cuticle secretion inhibits effectivestaining (CAMPOS-ORTEGA and HARTENSTEIN 1997 ). Thus, errantgerm cells persist in out mutants and continue to express thefaf-lacZ marker.

To determine whether this defect in cell death is linked toa migration defect, we determined the number and location ofgerm cells present in 11- to 12-hr embryos. The results arepresented in Table 3. Control embryos had an average of 13.7germ cells (n = 50) in the gonads compared to an average of13.0 germ cells in out¹/out¹ mutants (n = 50). These numbersare not statistically different (P = 0.16, Student's t-test).An average of 8.6 germ cells was observed ectopic to the gonadin the mutants, compared to 0.3 ß-Gal-positive germcells outside of the gonads in controls. The range was 4–18ectopic germ cells in the out mutants. The average total numberof germ cells in out¹/out¹ embryos is 21.6. This number is statisticallydifferent from the average of 14.0 observed in controls (P <0.0001, Student's t-test).

As an additional test of whether the Faf-ß-Gal-positivecells outside of the gonad are continuing to express the germcell fate, we analyzed the expression of Vasa-GFP, another germcell-specific marker (BREITWIESER et al. 1996 ). The Vasa-GFPgerm cell labeling pattern is indistinguishable from the Faf-ß-Galstaining pattern in out¹/out¹ embryos (data not shown). In addition,the Faf-ß-Gal-labeled cells are larger than neighboringcells and possess the distinct spherical nucleus typical ofgerm cells (RABINOWITZ 1941 ; POULSON 1950 ; UNDERWOOD etal. 1980 ). Therefore, the mislocalized cells in out/out embryoscontinue to display three independent germ cell traits. Thesedata suggest that mutations of the out gene disrupt the programmedcell death of the germ cells.

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

We report the identification of two X-linked genes, sctt andout. When mutated, sctt severely disrupts germ cell migration,and the germ cells ectopic to the gonad fail to undergo programmedcell death. The sctt mutant flies are often sterile, and thefemales have a high percentage of agametic ovaries. Zygoticexpression of a wild-type copy of sctt rescues germ cell migration,but not the germ cell death defect. Thus, the sctt mutationdisrupts at least two developmental processes: the pathfindingmechanisms that enable the germ cells to migrate to the gonadand the regulation of cell survival. In out mutant embryos,the same numbers of germ cells are incorporated into the gonadsas in wild-type embryos. Thus, germ cell migration is normal.However, germ cells ectopic to the gonads do not undergo programmedcell death. We propose two models for out function. The functionof out may be part of a cell death mechanism responsible forthe elimination of germ cells ectopic to the gonad. Alternatively,a mutation in out may result in increased activity of a survivalfactor that allows germ cells ectopic to the gonad to persist.

Maternal sctt regulates cell migration:
The sctt phenotype has several noteworthy features. First, itrequires that the mother be homozygous mutant. To date, onlythe products of the nos and pgc-1 genes are known to be requiredin the germ cells for normal migration (KOBAYASHI et al. 1996; NAKAMURA et al. 1996 ; FORBES and LEHMANN 1998 ). Both arematernally contributed. Mutation of pgc-1, an untranslatableRNA, results in decreased nos RNA levels after the cellularblastoderm stage. Therefore, the germ cell phenotype of pgc-1embryos may be the result of its effect on nos expression. Nos,a zinc-finger protein, is necessary to suppress transcriptionand mitosis in the germ cells (KOBAYASHI et al. 1996 ; ASAOKAet al. 1998 ; FORBES and LEHMANN 1998 ; DESHPANDE et al. 1999). Zygotic expression of nos does not rescue the germ cell migrationdefect (FORBES and LEHMANN 1998 ). Since the germ cell migrationdefect of sctt mutants can be rescued zygotically, sctt mayfunction in germ cell migration later than nos. In fact, thenos germ cell migration phenotype is clearly distinct from thesctt phenotype. Germ cells deprived of maternal nos expressionexit the posterior midgut and then cluster close to the posteriormidgut rudiment (FORBES and LEHMANN 1998 ). The sctt mutantgerm cells cross the midgut epithelium and disperse individuallythroughout the posterior of the embryo.

Since the germ cell migration phenotype of sctt mutant embryosis so severe, we favor the hypothesis that the agametic ovariesare caused by a failure of germ-line stem cells to populatethe gonads. A similar agametic ovary phenotype has been reportedfor wunen mutants (ZHANG et al. 1996 ). Paternal rescue of germcell migration and the concomitant restoration of fertilityby a wild-type copy of sctt are consistent with this interpretation.However, it is possible that the sctt mutation disrupts a laterdevelopmental event within the ovary, resulting in a degenerationof germ-line stem cells or a very early arrest of oogenesis.

It is likely that additional alleles of sctt were generatedin our screen, but they were not successfully retained. To observethe germ cell defects resulting from a mutation of sctt, a homozygousmutant female must be viable and fertile. Therefore, lethalor sterile chromosomes would not have been recovered. In addition,sctt males are only 33.7% fertile, and females are only 41.7%fertile. Homozygous viable lines may have been lost becauseof a failure to reproduce. Noncomplementation screens specificallydesigned to isolate additional alleles of sctt will be requiredfor a more thorough genetic analysis of the sctt locus.

Cell migration coupled to cell survival:
Another interesting feature of sctt is that it affects bothgerm cell migration and germ cell survival. However, the temporalrequirements for sctt in these two processes are different.The effect on germ cell death is not rescued by zygotic expressionof a wild-type copy of the gene. In some experimental systems,migration guidance cues have been shown to be integrally linkedto or to have additional functions as survival factors (FLEISCHMAN1993 ; GOETZL and AN 1998 ; KUNISADA et al. 1998 ; WAKAMATSUet al. 1998 ; ASHMAN 1999 ; DE FELICI 2000 ; GOETZL et al.2000 ; SWARTHOUT and WALLING 2000 ; FUKUSHIMA et al. 2001; KIERSZENBAUM and TRES 2001 ; MILLER and KAPLAN 2001 ). Forexample, in avian and mouse embryos, the receptor tyrosine kinase,c-Kit, and its ligand, Stem cell factor, have been shown toact as both cell migration and anti-apoptotic factors in bothneural crest and germ cell lineages (FLEISCHMAN 1993 ; KUNISADAet al. 1998 ; WAKAMATSU et al. 1998 ; ASHMAN 1999 ; DE FELICI2000 ; KIERSZENBAUM and TRES 2001 ). In neurons, neurotrophinscan act as both prosurvival and proapoptotic signals, dependingupon the developmental context and receptor configuration ofthe receiving cell (MILLER and KAPLAN 2001 ).

Recently, DESHPANDE et al. 2001 demonstrated that ectopicexpression of hedgehog could act as an attractive signal forDrosophila germ cells. In avian embryos, CHARRIER et al. 2001 have shown that Sonic hedgehog can act as an anti-apoptoticfactor in neural tube formation. Considering the proposed roleof Hedgehog as an attractive signal for germ cell migrationin Drosophila, it is possible that Hedgehog may be involvedin both pathfinding and cell survival in germ cell development.

The lysophospholipid class of molecules, including lysophosphatidicacid and sphingosine 1-phosphate, has been shown to mediateboth survival and cell migration behaviors (GOETZL and AN 1998; GOETZL et al. 2000 ; SWARTHOUT and WALLING 2000 ; FUKUSHIMAet al. 2001 ). In zebrafish, a sphingosine-1-phosphate receptorhas been shown to be necessary for heart precursor cell migration(KUPPERMAN et al. 2000 ). The recently identified roles of variouslipid-modifying enzymes in Drosophila germ cell migration, includinga phosphatidic acid phosphatase and 3-hydroxy-3-methylglutarylcoenzymeA reductase, make lipid-based signals likely candidatesfor germ cell guidance cues (ZHANG et al. 1996 , ZHANG et al.1997 ; VAN DOREN et al. 1998 ; STARZ-GAIANO et al. 2001 ).Overexpression of wunen can act at a distance to decrease germcell number (STARZ-GAIANO et al. 2001 ). Deciphering the potentialrole of the lysophospholipid class of signaling molecules incell migration and/or cell survival will be a particularly interestingarea of study.

It is possible that inappropriate cell division may contributeto the sctt and out cell death phenotypes. In nos mutant germcells and patched mutant embryos, germ cells reenter the cellcycle prematurely and the number of germ cells is increased(DESHPANDE et al. 1999 , DESHPANDE et al. 2001 ). Germ cellsectopic to the gonad are frequently observed in these embryos.However, the total number of germ cells we observe in out andsctt mutant embryos is less than that observed in either thenos or the patched mutant backgrounds. Other observations suggestthat the extra germ cells observed in the sctt and out mutantsare insufficient to override the embryo's ability to eliminatethese additional cells. When a 39% increase in germ cell numberis caused by the overexpression of osk in 6X osk embryos, ectopicgerm cells are not seen after gastrulation (SMITH et al. 1992). In our faf-lacZ genetic background, a mutation that causesa 29% increase in the number of germ cells forming at the posteriorpole does not result in an increase in germ cells ectopic tothe gonads (C. R. COFFMAN and R. E. BOSWELL, unpublished results).Therefore, the Drosophila embryo appears to have some additionalcapacity for destroying germ cells ectopic to the gonads, andthe generation of additional germ cells cannot completely accountfor the out and sctt phenotypes.

Programmed cell death and Drosophila germ cells:
There are multiple types of programmed cell death. Programmedcell death via apoptosis and autophagy has been reported inDrosophila (ABRAMS et al. 1993 ; FOLEY and COOLEY 1998 ; ABRAMS1999 ; BANGS and WHITE 2000 ; LEE and BAEHRECKE 2000 , LEEand BAEHRECKE 2001 ). While apoptosis and autophagy have distinctmorphologies, they utilize some of the same molecular machineryand therefore cannot always be distinguished using molecularmarkers.

Over 60 years ago, Drosophila biologists demonstrated that thenumber of primordial germ cells exceeds the number of germ cellsincorporated into the gonads (RABINOWITZ 1941 ; SONNENBLICK1941 ). These authors and others have suggested that this reductionin germ cell number is likely to occur via an active and highlyregulated process (SONNENBLICK 1950 ; TECHNAU and CAMPOS-ORTEGA1986 ; STARZ-GAIANO et al. 2001 ). However, a direct demonstrationof the cellular mechanism or mechanisms responsible for theelimination of these germ cells has not been reported. STARZ-GAIANOet al. (2001) make the interesting observation that forced expressionof Wrinkled [W, a.k.a. head involution defective (hid)] or reaper(rpr) in germ cells results in their death. This argues thatthe machinery for apoptotic or autophagic cell death is presentin the germ cells, as both of these programmed cell death mechanismsutilize W/hid or rpr functions (LEE and BAEHRECKE 2001 ; THUMMEL2001 ).

High levels of p53 RNA expression are observed in Drosophilaprimordial germ cells. This may reflect a function for thispro-apoptotic gene in the elimination of germ cells that haveexperienced DNA damage. In support of this hypothesis, p53 hasbeen shown to activate the expression of rpr, a cell death activator,in cells exposed to radiation-induced DNA damage (BRODSKY etal. 2000 ; OLLMANN et al. 2000 ). Determining whether the eliminationof germ cells ectopic to the gonad utilizes the caspase-mediatedpathways activated by the cell death inducers rpr, grim, sickle,and W (ABRAMS et al. 1993 ; ABRAMS 1999 ; BANGS and WHITE2000 ; LEE and BAEHRECKE 2000 , LEE and BAEHRECKE 2001 ; CHRISTICH et al. 2002 ; SRINIVASULA et al. 2002 ) or by somealternative cell death pathway such as the one reported fornurse cells (FOLEY and COOLEY 1998 ), will require further investigation.Future studies may also reveal roles for genes that affect theexpression and/or regulation of cell death inhibitors such asiap1/thread, iap2, or Deterin (ABRAMS 1999 ; VERNOOY et al.2000 ). None of the known cell death genes identified to datemap to the sctt or out regions.

The presence of a large number of germ cells outside of thegonads in both sctt and out mutants indicates that mutationsin these genes affect the elimination of these germ cells andthat the death of germ cells ectopic to the gonads occurs viaan active, developmentally regulated process. Both phenotypesare recessive, and in the case of out, germ cells ectopic tothe gonad are observed when out is placed over a deletion. Thisindicates that these out alleles are loss of function. However,we have not demonstrated whether apoptosis, autophagy, or someother mechanism of programmed death is disrupted in sctt andout mutants. We also cannot rule out the formal possibilitythat necrosis is responsible for some germ cell loss duringdevelopment. It has been proposed that the lost germ cells maylack sufficient germ plasm (SONNENBLICK 1950 ).

The germ cells of Drosophila are an excellent model for studyingcell death, and there is great potential for identifying additionalgenes necessary for this process. Since only $~$ 50% of the germcells successfully reach the gonad, $~$ 10–30 germ cells normallyundergo developmental cell death in the embryo (SONNENBLICK1941 , SONNENBLICK 1950 ; UNDERWOOD et al. 1980 ; TECHNAUand CAMPOS-ORTEGA 1986 ).

Mutations that affected germ cell survival occurred very frequentlyin our screen. There are at least two explanations for this.First, the ability to detect germ cells outside the gonad isrequisite for a screen like the one reported here. If the "lost"germ cells immediately ceased expression of germ cell-specificmarkers, then the phenotype of a germ cell migration defectivemutant would be a reduction in the number of germ cells withinthe gonad and might go undetected. Therefore, our screen wasvery effective at identifying mutations that affect germ celldeath as well as germ cell migration.

Second, the mechanisms regulating germ cell survival and deathare likely to have many components. Therefore, there are manypotential targets for mutagenesis screens. Since very few geneshave been identified with roles in Drosophila germ cell migrationand death, additional screens will be required to achieve amore complete understanding of these processes. In addition,it will be interesting to examine potential cell death defectsin other germ cell migration mutants identified and to investigatepossible interactions between these genes and sctt and/or out.Further, it will be important to determine whether sctt andout function in the same pathway or in distinct pathways toregulate germ cell survival.

ACKNOWLEDGMENTS

We thank Janice Fischer, Joseph Heilig, Linda Ambrosio, JosephDuffy, and the Bloomington and Umeå stock centers forproviding the Drosophila stocks used in this work. Jo Anne Powell-Coffman,Kristen Johansen, William Nordstrom, Angela Mortvedt, and CorinneGlynn provided critical comments on the manuscript. C.R.C. wassupported by a Howard Hughes Medical Institute postdoctoralfellowship at the University of Colorado where the initial phasesof this work were performed. The genetic and phenotypic analysesof out and sctt were conducted at Iowa State University andwere supported by funds provided to C.R.C. by the Iowa Agricultureand Home Economics Experiment Station. R.E.B. is funded by NationalInstitutes of Health grant GM-57989. This manuscript, designatedas J-19748 of the Iowa Agriculture and Home Economics ExperimentStation, Ames, Iowa, project no. HIOW03383, was supported byHatch Act and State of Iowa funds.

Manuscript received February 21, 2002; Accepted for publication June 21, 2002.

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