Institut Jacques Monod, UMR 7592 CNRS/Université Pierre et Marie Curie/Université Denis Diderot, Laboratoire de Génétique du Développement et Evolution, 2-4 place Jussieu, 75251 Paris Cedex 05, France
*Author for correspondence (e-mail: pret{at}ijm.jussieu.fr)
Accepted 2 June 2002
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SUMMARY |
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Key words: Oogenesis, Intercellular signaling, Prefollicular cells, Morphogenesis, Cell-cell adhesion, Drosophila
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INTRODUCTION |
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In the Drosophila ovary, each oocyte develops inside an independent follicle also termed egg chamber. Egg chambers are formed in the anterior part of the ovariole, the germarium and mature progressively towards the posterior part of this autonomous unit of the ovary. The germarium has been divided into three distinct subregions according to morphological criteria. Anterior region 1 contains two to three germline stem cells (GSCs) identified by clonal analysis (Wieschaus and Szabad, 1979) and laser ablation studies (Lin and Spradling, 1993
), and marked by the presence of a spherical cytoplasmic structure called the spectrosome (Lin et al., 1994
). GSC division is asymmetric and generates both a daughter stem cell and a differentiated daughter cell called a cystoblast. Each cystoblast undergoes four rounds of mitosis with incomplete cytokinesis to produce a syncytium of 16 cystocytes known as a germline cyst. Complete cysts then mature through region 2a and become enveloped individually in region 2b by inwardly migrating somatic cells (or prefollicular cells) deriving from approx. two somatic stem cells (SSCs) lying at the border between regions 2a and 2b (Margolis and Spradling, 1995
). The prefollicular cell population diverges soon after to give rise to interfollicular stalk cells (which individuate egg chambers), two pairs of polar cells (which mark anterior and posterior poles of the egg chamber) and follicular cells (which form a polarized epithelium around each egg chamber). Germline sister cells acquire different cell fates too, as in each cyst one single cell is determined to become the oocyte, while the 15 remaining cells will differentiate as nurse cells. Region 3 of the germarium corresponds to a stage 1 egg chamber (Spradling, 1993
) that will bud off upon completion of stalk formation.
Egg chamber formation is thus a sequential process that requires coordination between somatic and germline differentiation programs, probably mediated by intercellular signaling between these two cell lineages. Although somatic cell differentiation in the germarium is a key step in this process, small cell size, intermingling between proliferation, migration and early differentiation events, and lack of specific early markers have impeded the precise elucidation of the prefollicular cell differentiation program. Nonetheless, at least three crucial steps in prefollicular cell maturation are evident. Region 2a/2b prefollicular cells first specifically recognize mature 16-cell cysts and individuate them via morphogenetic events involving projections of cellular processes and probably also migration per se. In the absence of germline cells, prefollicular cells do not undergo any cell shape changes (Spradling et al., 1997). In addition, both secreted proteins (Brainiac, Egghead, Gurken/TGF-
) encoded by genes with germline specific function and transmembrane proteins expressed in prefollicular cells (Torpedo/EGFR) are thought to act as components of germen to soma signaling pathways required for correct encapsulation of mature 16-cell cysts by prefollicular cells (Goode et al., 1996a
; Goode et al., 1996b
; Goode et al., 1992
; Rubsam et al., 1998
). Region 2b intercyst cells then gain specific adherence properties: they accumulate DE-Cadherin and attract the oocyte posteriorly, thereby polarizing the egg chamber. This posterior positioning of the oocyte is mediated by homophilic interactions as DE-Cadherin function is required in both germline and somatic cells for this sorting-out process (Godt and Tepass, 1998
; Gonzalez and St Johnston, 1998
). Last, cell lineage divergence among prefollicular cells takes place in region 2b/3, allowing specification of polar cells, stalk cells and follicular cells. Recently, germen to soma Delta/Notch signaling has been shown to be required for polar cell differentiation (Grammont and Irvine, 2001
; Lopez-Schier and St Johnston, 2001
). Lack of Notch, Fringe or Suppressor of Hairless in somatic cells, or of Delta in germline cells leads to an absence of polar cells. This is coupled with defective egg chamber individuation and abnormal stalk assembly, revealing the key role played by polar cells in early egg chamber formation.
The fused (fu) gene has been identified as a positive effector of the Hedgehog (Hh) signal transduction pathway in Drosophila embryonic and imaginal disc development (Alves et al., 1998; Ingham, 1993
; Limbourg-Bouchon et al., 1991
; Sanchez-Herrero et al., 1996
). Although, previous analysis has revealed that fu mutations are associated with reduced female fecundity (Busson et al., 1988
) and loosely characterized ovarian tumors (King, 1970
), fu function in oogenesis has not been clearly defined. The fu gene encodes a serine/threonine kinase that can be subdivided into two domains, an N-terminal catalytic domain and a C-terminal putative regulatory region (Therond et al., 1996
). However, no substrates for Fu kinase activity have been identified in any system. Several Fu partners in Hh signal transduction have been characterized in the embryo and wing imaginal disc: the transmembrane proteins Patched (Ptc) and Smoothened (Smo); and cytoplasmic proteins belonging to a multiprotein complex, namely Costal2 (Cos2), Suppressor of fused (Sufu), Cubitus interruptus (Ci) and Fu itself (reviewed by Murone et al., 1999
). Genetic and molecular studies have led to a model in which binding of Hh to Ptc releases inhibition of Smo activity, which generates modifications in the properties of the regulatory cytoplasmic complex and, finally, results in the activation of the transcription factor Ci and subsequent transcription of target genes. In the ovary, Hh is secreted by anterior terminal filament cells and is required for SSC maintenance and proliferation (Forbes et al., 1996a
; Zhang and Kalderon, 2001
). Known components of the Hh signaling pathway are present in the ovary in addition to Hh [Ptc (Forbes et al., 1996b
), Smo (F. B. and A.-M. P., unpublished), Cos2 (Vied and Horabin, 2001
) and Ci (Forbes et al., 1996b
)] and their activity is required in SSCs to regulate Hh signal transduction and, therefore, SSC proliferation (Zhang and Kalderon, 2000
; Zhang and Kalderon, 2001
). To date, no early function in prefollicular cell patterning has been clearly demonstrated for cytoplasmic transducers of Hh signaling.
We have undertaken an analysis of the fu mutant ovarian phenotype and report on the characterization of defects associated with ovarioles producing multicyst (two to several) and apposed egg chambers exhibiting advanced nurse cell and oocyte development. Our characterization of the fu so-called tumorous egg chamber phenotype will be presented elsewhere (F. B. and A. M. P., unpublished). Our analysis reveals that fu is required for at least three aspects of prefollicular cell morphogenesis during egg chamber formation: (1) prefollicular cell migration around germline cysts; (2) prefollicular cell intercalation during interfollicular stalk formation; and (3) posterior oocyte positioning in the egg chamber. Although we show that fu is expressed in both germline and somatic cells from the germarium onwards, clonal analysis demonstrates cell autonomous action of fu in prefollicular cells for all three aspects of proper egg chamber formation mentioned above. In contrast to other classical components of Hh signal transduction, we show that fu does not play a role in SSC proliferation. However, genetic interaction studies and the analysis of the effects of reduced Hh signal transduction in the ovary indicate that fu acts in the classical genetic pathway for Hh signal transduction in the ovary and that fu-dependent Hh signaling plays a role in prefollicular cell differentiation. This study therefore reveals that soma to soma signaling, in addition to soma-to-soma signaling, is necessary for prefollicular cells to adopt their characteristic dynamic morphogenetic properties.
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MATERIALS AND METHODS |
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The ptc-lacZ (Alves et al., 1998), ptc-Gal4 (Bloomington Stock number 2017), hs-hh (Tabata and Kornberg, 1994
), Sufu LP (Préat, 1992
), cos2WI/CyO (Sisson et al., 1997
), hhts2/TM6 and hhAC/TM3 (Ma et al., 1993
) strains were used to test for a role of the Hh pathway. UAS-cos2/TM3 (K. Ho and M. Scott, unpublished) and UAS-Cicell (189.2) (Methot and Basler, 1999
) were used for flip-out/Gal4 clonal analysis. Cicell encodes a truncated form of Ci shown to act as a constitutive transcriptional repressor (Methot and Basler, 1999
).
The 93F and A101 enhancer-trap lines (Bier et al., 1989; Ruohola et al., 1991
) were used for tissue-specific ß-galactosidase staining in interfollicular stalks and polar cells, respectively.
In our experiments, wild-type reference females correspond to fu heterozygous females that originate from the same line or cross as fu homozygous sisters, except in the case of fu in situ hybridization and immunodetection experiments for which the Oregon R strain was used.
Egg chamber staining procedures
Immunocytochemistry was performed as described (McKearin and Ohlstein, 1995). The following antibodies were used in this study: mouse monoclonal anti-Orb 6H4 (1:30; Developmental Studies Hybridoma Bank [DSHB]), mouse monoclonal anti-Fas III 68BAC11 (1:30; Y. N. Jan, unpublished), rabbit anti-
-Spectrin (1:1000) (Byers et al., 1987
), rat monoclonal anti-DE-Cadherin (1:20) (Oda et al., 1994
), mouse monoclonal anti-Hts 1B1 (1:5; DSHB), rabbit polyclonal anti-Fu (1:200) (Robbins et al., 1997
) and rabbit polyclonal anti-ß-galactosidase (1:200; Boehringer). All the fluorescence-conjugated secondary antibodies were purchased from Jackson Immunoresearch Laboratories and used at a 1:200 dilution. Actin was labeled with rhodamine-conjugated phalloidin (Molecular Probes) at 0.1 µg/ml for 20 minutes in PBS. All samples were mounted in cytifluor (Kent).
For DAPI staining, tissues were fixed in 4% formaldehyde in phosphate-buffered saline (PBS) for 30 minutes and rinsed twice, first in PBS with 0.1% Tween-20, then in PBS alone. Ovaries were placed for one night in PBS: glycerol (1:3), with 1 µg/ml of DAPI. ß-galactosidase activity detection was performed as described (Grammont et al., 1997). Whole-mount in situ hybridization was performed as described previously (Doerflinger et al., 1999
). Digoxigenin-labeled sense and antisense RNA probes for fu were synthesized from the D6 vector (Therond et al., 1999
), using the RNA genius kit (Boehringer Mannheim).
Samples were examined either with a Leica DMR microscope or by confocal microscopy using a Leica DMR-BE microscope.
Clonal analysis
For analysis of fuG3 and fuJB3 alleles, FRT-mediated recombination events were induced in SSCs with an e22c-Gal4, UAS-flp line (Duffy et al., 1998) and revealed by loss of constitutively expressed lacZ from a tub-nlslacZ reporter construct (Goode and Perrimon, 1997
). FRT19A nls-tublacZ/Y; e22c-Gal4 UAS-flp/+ males were mated to FRT19A fuX/FM6 females to produce FRT19A fuX/ FRT19A tub-nlslacZ; e22c-Gal4 UAS-flp/+ females (fuX denotes either fuJB3 or fuG3). From the moment of the cross onwards, flies were kept at 25°C and dissected about 8 days after eclosion. For the fumH63 allele, y w hsp-flp fumH63; FRT40A P[fu+] arm-lacZ/FRT40A P[y+] females were generated as described (Zhang and Kalderon, 2000
). Flipase expression was induced by heat-shocking third instar larvae at 38°C for 1 hour. Dissection of 8- to 10-day-old females ensured that observed clones corresponded to stem cell clones.
Flip-out/Gal4 clones were produced by mating hsp-flp; UAS-Cicell/SM6-TM6 or hsp-flp; UAS-Cos2/SM6-TM6 males with Act>CD2>Gal4 UAS-GFP females (Neufeld et al., 1998; Pignoni and Zipursky, 1997
) and heat-shocking late pupae at 37°C for 1 hour. Flies were thereafter kept at 25°C and dissected about 8 days after eclosion. Clones were marked by GFP staining.
Hh overexpression
To express Hh ectopically, we used a hs-hh transgene in which the hh-coding sequence has been placed under the control of the hsp70 promoter (Tabata and Kornberg, 1994). One-day-old flies were heat-shocked for 2 hours at 38°C and dissected and treated for X-gal staining 3 days later.
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RESULTS |
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In many fu mutant germaria, some prefollicular cell migration between germline cysts was evident, but the dynamics of Fas III expression in these cells, their morphology and subsequent encapsulation were all abnormal. Once again, the long, thin prefollicular cell processes containing Fas III were largely absent (Fig. 2C,D). Prefollicular cells exhibiting strong Fas III staining were observed that had migrated between germline cysts, but these cells were often somewhat cuboidal, showing more lateral than apical Fas III staining, irregular encapsulation of cysts and limited intercalation for stalk formation (Fig. 2C,D, arrows). In addition, cells staining weakly for Fas III were found grouped together at the exterior of germaria or of newly formed chambers (Fig. 2C,D, asterisks), which may represent abortive stalk formation.
Even under these unfavorable circumstances, some egg chamber budding does occur (Fig. 2D). Interestingly, when newly formed multicyst chambers were observed (>16 germ cells, Fig. 2D'), they showed internal compartmentalization by somatic cells weakly staining for Fas III (Fig. 2D, open arrowhead). These cells have not intercalated to form a stalk, nor have they formed a follicular epithelium. Multicyst chambers of this type were present in-the-making in region 3 of the germarium (Fig. 2C, open arrowhead, C'), which may be eventually budded off by more anterior prefollicular cells that stain strongly for Fas III (Fig. 2C, arrow). More posteriorly in the ovariole, this partitioning of multicyst egg chambers by somatic cells was not observed, suggesting that these cells may be eventually degraded (data not shown). Therefore, defective prefollicular cell behavior in region 2b of fu mutant germaria (Fig. 2B-D) is probably what leads to the inclusion of several cysts in one chamber.
fu mutant ovarioles exhibit abnormal interfollicular stalk formation
In order to look at interfollicular stalk cell specification, we used the 93F enhancer trap line, which expresses the lacZ gene specifically in these cells once stalk morphogenesis is complete (Fig. 3A', insert, for ß-galactosidase immunodetection and C', insert, for X-Gal staining). Concomitant to 93F upregulation in interfollicular stalks, Fas III expression diminishes significantly (Fig. 3A,A', insert). In fu mutant germaria that exhibit egg chamber budding defects, we found small, peripheral groups of cells expressing both low levels of Fas III compared with neighboring prefollicular cells (Fig. 3B, arrow, see also Fig. 2C,D, asterisks), and the 93F interfollicular stalk cell marker (Fig. 3B', insert). Therefore, these stalk cells appear to be specified as such, but they are set aside, unable to fulfill their role in budding off of individual egg chambers. In addition, we found that stalk-like structures between egg chambers in fu mutant ovarioles express the 93F stalk cell marker, although these stalks exhibit an abnormal morphology. Instead of presenting the wild-type linear arrangement of five to seven oval-shaped cells (Fig. 3C', insert), fu mutant stalks were comprised of aggregates of round cells arranged in a ball shape (Fig. 3D', insert). Therefore, fu mutations do not appear to affect stalk cell specification, at least with respect to the 93F marker, but rather their morphogenetic properties during egg chamber budding.
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We also examined the expression of the cell-cell adhesion protein, DE-Cadherin, which has been shown previously to be polarized apically in prefollicular cells during egg chamber budding (Fig. 3G,G'). By examining expression of this protein in many wild-type germaria, with the intention of visualizing all stages of egg chamber budding, including those that may occur rapidly, we identified a transition in the expression pattern of DE-Cadherin in pre-stalk cells that seems to correspond to the initiation of intercalation between these cells. First, prefollicular cells that have displaced themselves centripetally between germline cysts make apical cell-cell membrane contacts that accumulate DE-Cadherin specifically (Fig. 3G', bracket). The staining is observed as two apical bands separated by a space suggesting that these cells first make contacts with adjacent cells rather than opposing cells. Although the nuclei of these cells have moved centripetally they are not fully apical as yet. In what appears to be a subsequent step, as pinching off of the stage 1 egg chamber by pre-stalk cells has progressed further (Fig. 3I), DE-Cadherin expression changes dramatically (Fig. 3I', bracket). It appears as an apical zig-zag expression pattern that probably corresponds to new lateral surface contacts established upon intercalation between these cells. The nuclei of these cells are now also positioned more apically and their appearance by DAPI staining is more diffuse than before, perhaps in preparation for the intercalation process. In contrast to wild-type animals, in fu mutants, a high proportion of germaria displayed the pre-intercalation arrangement of pre-stalk cells, these cells expressing strong apical DE-Cadherin (Fig. 3H,H'), while the initiation of intercalation, characterized by a zig-zag DE-Cadherin expression pattern, was largely absent. These results suggest that pre-stalk cells in fu mutants are compromised in their ability to initiate the intercalation process, which would lead to delayed egg chamber budding. However, apical polarization of DE-cadherin is not affected in fu mutant pre-stalk cells (Fig. 3H'). In fact, even in fu mutant germaria in which prefollicular cells have not completed their centripetal migration between germline cysts, DE-Cadherin is nonetheless expressed and localized apically (Fig. 3J,J'). It is possible that DE-Cadherin accumulation is somewhat excessive in fu mutant pre-stalk cells compared with wild type, in particular in those cells that are in contact with the germline (compare Fig. 3G' with 3H' and data not shown). However, these experiments do not allow us to determine whether this excess apical accumulation is the cause of delayed intercalation or rather the result.
Given that stalk cells and polar cells are closely linked by lineage (Tworoger et al., 1999), we also looked at polar cell specification in fu mutants using anti-Fas III antibodies and the A101 enhancer trap line. In wild-type ovaries, these two markers are expressed in polar cell pairs at each pole of the egg chamber, as of the stage 2 egg chamber, which is fully budded from the germarium (Fig. 3E', insert). In relatively young fu mutant females, the first egg chamber that fully buds off the germarium also expresses these polar cell markers appropriately (Fig. 3F', insert); however, this egg chamber is considerably older than the stage 2 egg chamber expressing these markers in wild-type ovarioles. Therefore the delay in stalk formation in fu mutants is also accompanied by a delay in polar cell specification. In older fu mutant females, which contained multicyst and apposed types of egg chambers, several pairs of cells expressing the Fas III and A101 polar cell markers were observed, with a good correlation between the number of germline cysts in these chambers and the number of pairs of polar cells (data not shown). Finally, polar cell specification occurs in fu mutant clones induced in somatic stem cells and their descendents using several fu alleles, including the pupal lethal strong hypomorphic allele, fumH63 (see below and Fig. 5A', insert). Therefore, fu is not required for either stalk or polar cell specification.
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In addition, long, disorganized stalks were observed (Fig. 5C,C', arrows) from which egg chambers showed an off center attachment. Interestingly, in the great majority of cases observed, these stalks were composed of fu+ cells, while fu mutant cells were found as part of the follicular epithelium of the adjacent chambers (Fig. 5C'). We next examined germarial regions 2b/3 more closely and observed that segregation of fu+ and fu cells already occurs at this point. fu+ prefollicular cells were observed that had migrated centripetally over a germline cyst (Fig. 5D,D', asterisks), while adjacent fu prefollicular cells remained at the periphery (Fig. 5D,D', arrows). fu cells thus appear compromised in their capacity to migrate over germline cysts, and the asymmetric budding by fu+ cells is probably what leads to the generation of abnormally shaped and mispositioned fu+ stalks. The differential capacities of fu+ and fu cells were also observed in rare mosaic stalks where fu and fu+ cells were present together (Fig. 5E,E'). Both fu and fu+ stalk cells take on a flattened shape but do not intercalate, remaining as two independent stacks of cells instead. These results indicate that fu function is necessary in prefollicular cells in order for them to acquire adhesive and/or migratory properties, allowing them to encapsulate germline cysts and intercalate.
fu mosaic egg chambers contain mislocalized oocytes
Competition between fu and fu+ cells generated in mosaic ovarioles revealed an additional property of fu prefollicular cells, as mosaic ovarioles were shown to contain chambers with perturbed anteroposterior asymmetry. Indeed, although the oocyte is invariantly found at the posterior pole of wild-type egg chambers, mosaic epithelia were often associated with a mislocalized oocyte, as revealed by anti-Orb immunostaining (compare Fig. 6A-A'' with 6B,B' arrows). Strikingly, we noticed that the position of the misplaced oocyte is not random, since mislocalized oocytes orient themselves with high fidelity towards fu+ cells (82.5%, n=40), independently of where these cells are located. In particular, laterally (Fig. 6A-A''), as well as anteriorly localized oocytes (data not shown) could be found. Therefore, this observation indicates a failure of posterior fu follicle cells either to drive early oocyte sorting out or to maintain the posterior position of the oocyte. As posterior localization of the oocyte has been shown to occur at the transition from germarial region 2b to region 3 in wild-type ovaries (Godt and Tepass, 1998; Gonzalez and St Johnston, 1998
), we next examined germaria of mosaic ovarioles and found that oocytes were already mispositioned as of this stage (Fig. 6C,C', arrows). In addition, similar defects in early posterior positioning of the oocyte are observed in fu mutant females (data not shown), though less frequently than in mosaic ovarioles where fu and fu+ cells are in competition. These results therefore suggest that removing fu function in prefollicular cells prevents oocytes from correctly reaching the posterior of germline cysts.
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Somatic stem cell clones were generated using three different fu alleles including the strong hypomorphic fumH63 allele. No significant difference in the frequency or in the size of clones was observed between fu and control stem cell clones generated in parallel according to a chi-square test (Table 1, =0.15). Even in 8- to 10-day-old females, fu mutant cells were typically found spread throughout mosaic ovarioles (Figs 5, 6, and data not shown), suggesting that neither SSC nor follicular cell division rates are affected in fu mutant ovarioles.
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With this aim in view, we tested whether fu mutations could affect the transcription of ptc, a classical Hh target gene. For this, a ptc-lacZ enhancer trap expressed in the same cells as endogenous ptc in embryos and in the stripe of strongest ptc expression in wing discs (Alves et al., 1998) was used. In the ovary, ptc-lacZ is expressed in a subset of ptc-expressing cells (anterior somatic cells) (Fig. 7A). This construct is responsive to variations in Hh levels since a strong increase in ptc-lacZ expression is observed after ectopic induction of hh using a hs-hh transgene (Fig. 7B). Strikingly, this ectopic transcription does not occur in a fu mutant context (Fig. 7C). In fact, even basal ptc-lacZ expression was abolished in fu females, which was confirmed using another P-element reporter (ptc-Gal4) also inserted in the ptc locus (data not shown). Therefore, fu seems to be necessary downstream of hh for the activation of this ovarian somatic ptc enhancer.
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We then asked whether overexpression of wild-type Ci could at least partially restore fu ovarian phenotypes, as is the case for the fu wing phenotype (Alves et al., 1998). Using the flip-out/Gal4 system, we generated ovarioles exclusively composed of Ci-overexpressing somatic cells (see Materials and Methods). These ovarioles did not exhibit any obvious defects (Table 3). However, somatic Ci overexpression significantly rescued fu ovarian phenotypes, as fuJB3 hsp-flp /fuJB3; UAS-Ci/+; Act-Gal4 UAS-GFP/+ females exhibited a higher proportion of normal ovarioles compared with their fuJB3 hsp-flp/fuJB3; SM6/+; Act-Gal4 UAS-GFP/TM6 sisters (Table 3).
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Reducing Hh signaling phenocopies fu ovarian phenotypes
This is the first time that a loss-of-function study unambiguously reveals a role for components of the Hh signal transduction pathway in somatic cell differentiation and egg chamber formation. Indeed, removing the function of Smo and Ci, two positive Hh signal transducers, results in a strong and early block in SSC proliferation, therefore hindering clonal analysis and interpretation of induced phenotypes. In order to circumvent this problem and to confirm this new function of Hh signaling, we tested several other genetic contexts allowing a partial reduction in Hh signaling. We first generated females with hypomorphic combinations of hh alleles (hhts2/hhts2 and hhAC/hhts2) and examined their ovarioles 4-5 days after shifting them to the restrictive temperature (29°C). As previously reported (Forbes et al., 1996a), we observed several ovarian defects including germaria exhibiting disorganized encapsulation (Fig. 8A) and multicyst egg chambers (Fig. 8B). However, such phenotypes cannot be solely interpreted as resulting from a deficit in somatic cell number as we found large groups of disorganized somatic cells, resembling those found in fu mutant ovarioles, at the periphery of hh mutant germaria and multicyst egg chambers (Fig. 8A',B', arrows). This suggests that hh mutant prefollicular cells are also defective in their capacity to migrate, individuate germline cysts and intercalate to form normal stalks.
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Altogether, our results are consistent with the existence of an ovarian fu-dependent Hh signaling pathway directly involved in prefollicular cell morphogenesis during egg chamber formation.
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DISCUSSION |
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Germline cyst encapsulation requires extension of cellular processes by prefollicular cells in regions 2a/2b of the germarium, such that they can recognize and adhere to mature 16-cell germline cysts, and subsequently migrate centripetally between individual cysts. Interfollicular stalk formation requires that pre-stalk cells in regions 2b/3 lose heterotypic adhesion to germline cells and gain homotypic adherence and the capacity to intercalate (Tworoger et al., 1999). The effector molecules implicated in these processes have not been characterized to a great extent, though several surface membrane and cytoskeletal proteins that have been shown to exhibit dynamic expression patterns in prefollicular cells and their descendants are likely to be involved. For example, several proteins (actin, Fas III, Hts,
-Spectrin, Filamin and others) are localized specifically to the cellular processes that prefollicular cells extend over germline cysts, and most of these are subsequently concentrated apically in pre-stalk cells just before their intercalation. Once the interfollicular stalk is formed, the expression of some of these proteins is downregulated in stalk cells (Fas III), while other proteins are expressed laterally in these cells (actin, Hts,
-Spectrin and PS1-ß integrin) (Gonzalez and St Johnston, 1998
; Lin et al., 1994
; Niewiadomska et al., 1999
; Ruohola et al., 1991
; Tanentzapf et al., 2000
; Zarnescu and Thomas, 1999
). Finally, proper expression of the DE-Cadherin, Armadillo/ß-Catenin and
-Catenin cell-cell adhesion complex at the membrane of both the posterior follicle cells and the oocyte probably mediates contact between these two cell types and posterior positioning of the oocyte (Godt and Tepass, 1998
; Gonzalez and St Johnston, 1998
).
We show here that, in fu mutant ovarioles, encapsulation of multiple cysts in a single egg chamber is associated with absence of prefollicular cell extensions around germline cysts and impaired centripetal migration of these cells. In addition, stalk formation in fu mutants is, in less affected individuals (young females with normal egg chambers), slow/delayed and, in more severely affected individuals (older females with multicyst egg chambers), very irregular (leading to abnormal stalk morphology). By following the expression of DE-Cadherin, which marks the apical membrane of pre-stalk cells, we show that, in fu mutants, pre-stalk cells that have migrated centripetally between germline cysts are blocked before the intercalation process. Induction of fu mutant clones in prefollicular cells led to the same types of encapsulation and stalk morphogenesis defects, indicating cell autonomous function in these cells for these processes. This study highlighted the impaired ability of fu mutant prefollicular cells to migrate between germline cysts and to participate to interfollicular stalk formation. This mosaic analysis also showed that fu mutant and wild-type cell populations have a tendency to remain segregated, implying that surface differences between these cells prevent their intermixing. Finally, fu function in prefollicular cells is implicated in another process involving specific cell-cell interactions, posterior positioning of the oocyte in the egg chamber. Taken together, these results suggest a function for fu in prefollicular cells for appropriate expression of one or several surface membrane or cytoskeletal proteins necessary for several aspects of prefollicular cell morphogenesis during egg chamber formation. Although we examined the expression of a number of cytoskeletal and membrane proteins in prefollicular cells in fu mutants (for example, DE-Cadherin, Fas III and others; data not shown), so far it has not been possible to relate the anomalies observed to a loss in expression or in polarized localization of any of these proteins. Interestingly, fu and other components of Hh signal transduction have been implicated in other developmental processes that involve establishing dynamic and differential cell-surface properties. For example, proper migration of germ cells during embryogenesis and their coalescence with somatic gonadal precursor cells to form the primitive gonad involves Hh expression in these somatic cells and function of components of classical Hh signal transduction in the germ cells (Deshpande et al., 2001). Dahmann and Basler (Dahmann and Basler, 2000
) also showed that opposing outputs of Hh signaling play a role in establishing differential cell affinities and thereby defining the anteroposterior compartment boundary in wing imaginal discs. This study also demonstrated that a difference in the level of DE-Cadherin expression alone was sufficient to maintain two wing disc cell populations segregated. However, the actual cell adhesion effectors that may be regulated by differential Hh signal transduction in wing development, as is the case for germ cell migration and egg chamber formation, remain to be determined.
Fu-independent Hh signal transduction in SSCs controls their proliferation
In the ovary, Hh signals from the terminal filament and cap cells and is required for SSC proliferation and subsequently for egg-chamber budding (Forbes et al., 1996a; Forbes et al., 1996b
). SSC self-renewing properties are not maintained in the absence of Hh signaling, whereas excessive Hh signaling produces supernumerary stem cells (Zhang and Kalderon, 2001
). In addition to the membrane receptors Ptc and Smo, Ci has been implicated in this process as a component of Hh signal transduction. However, in a hh loss-of-function context, SSC proliferation is restored by induction of low levels of somatic Hh signaling in SSC (achieved by removing protein kinase A function, an inhibitor of Ci activity, in these cells) (Zhang and Kalderon, 2000
). The authors therefore suggested that, as in wing imaginal disc development, where fu activity is required for transducing high but not low levels of Hh signaling, fu activity may not be endogenously required for regulation of SSC division (Alves et al., 1998
; Sanchez-Herrero et al., 1996
; Vervoort et al., 1999
). Our results obtained upon induction of fu mutant clones, as well as the quantitation of the mitotic activity of somatic cells in fu mutant germaria, confirm that fu is not necessary for SSC proliferation, suggesting that Hh signals to SSC through a Fu-independent pathway.
Fu-independent Hh signal transduction has already been reported in other systems (Suzuki and Saigo, 2000; Therond et al., 1999
). In the ventral ectoderm of the embryo, for example, Hh is secreted in a single row of cells at the parasegmental boundary and signals in both anterior and posterior directions, leading to the expression of the ptc gene in all neighboring cells. Interestingly, unlike smo and ci, fu function is required solely in anterior cells to transduce Hh signaling (Therond et al., 1999
). In the embryo as well as in the ovary, the differential requirement of Fu kinase activity can be interpreted either as a differential sensitivity of cells to Hh signal intensity and/or of target genes to Ci activation levels, or as the existence of position-specific modulators or even effectors of Hh response. Use of unconventional transducers has already been suggested for Hh signal transduction in posterior compartment cells of the wing imaginal disc (Ramirez-Weber et al., 2000
), Boldwigs organ cells (Suzuki and Saigo, 2000
) and ovarian germline cells (Vied and Horabin, 2001
).
Fu-dependent Hh signal transduction in prefollicular cells regulates egg chamber production
Our study reveals that fu endogenous function is required in prefollicular cells for acquisition of specific morphogenetic properties (see above). In addition, we provide several lines of evidence for a role for fu in a classical Hh signal transduction pathway within prefollicular cells for their participation to egg chamber formation. First, fu and hh mutant ovarian phenotypes overlap as both result in aberrant somatic cell behavior and formation of multicyst and apposed egg chambers (this study) (King, 1970). Second, fu is necessary, downstream of hh, for the expression of an ovarian somatic ptc-lacZ enhancer-trap. Third, fu ovarian phenotypes can be partially suppressed by removing either one or two copies, respectively, of two negative regulators of Hh signaling [Cos2 and Su(fu)], or by overexpressing the transcription factor Ci. Last, the morphogenetic defects described for fu mutant prefollicular cells can be phenocopied by somatic overexpression of either Cos2 or the inhibitory Cicell proteins. We therefore propose a model in which Hh signals at least twice in germarial somatic cells: first, through a fu-independent pathway to control SSC proliferation; and second, through a classical fu-dependent pathway to regulate early aspects of prefollicular cell differentiation. Therefore, fu loss-of-function mutations, which we show only affect prefollicular cell morphogenesis, allow the analysis of the role of Hh signal transduction in this process specifically.
Interestingly, previous studies focusing mostly on the effects of excessive Hh signal transduction in the ovary also indicated that two different stages of somatic ovarian cell development in the germarium are targeted by this signaling molecule (Zhang and Kalderon, 2000): early on (region 2a/2b), SSC proliferation and oocyte posterior positioning are affected; and later (region 2b/3) there is an apparent delay in the prefollicular cell development program, which, when combined with early effects on SSC proliferation, leads to the formation of giant stalks comprising poorly differentiated prefollicular cells between early egg chambers, delayed polar cell specification (stage 4 instead of 2) and an excess of these cells, and continued follicular epithelial cell division after stage 6. In fu mutants there is no effect on SSC or follicular cell proliferation, but some of the defects affecting prefollicular cells are similar, including non-posterior oocyte positioning, delayed prefollicular cell differentiation leading to delayed egg chamber budding and delayed polar cell specification. In addition, both somatic fu and ptc mutant clones show striking segregation from wild-type cells, fu mutant clones preferentially localized to the follicular epithelium, whereas ptc mutant clones localized to the stalks. These results indicate that cellular differences in Hh signal transduction levels, whether reduced (fu) or increased (ptc) compared with wild-type levels, affect the cell-cell recognition and adhesive properties of prefollicular cells. Taken together, these studies show that there is an overlap between the ovarian phenotypes associated with a reduction and an increase in Hh signaling, indicating that crucial levels of Hh signaling are required for prefollicular cell morphogenesis.
Nonetheless, fu mutations do not completely arrest egg chamber budding, rather causing a delay in several aspects of the prefollicular cell developmental program, including stalk and polar cell specification. Even fu mutant clones induced in prefollicular cells using the strong hypomorphic allele, fumH63, did not provoke more severe anomalies than the other alleles used in this study. These results suggest that prefollicular cell development does not depend solely on fu-dependent Hh signaling and that there is possibly some redundancy in the regulation of this process. Indeed, other studies have shown the importance of germline-emitted signals, in particular the secreted molecules Egghead, Brainiac and Gurken/TGF, for the encapsulation of germline cysts by prefollicular cells (Goode et al., 1996a
; Goode et al., 1996b
; Goode et al., 1992
; Rubsam et al., 1998
). In addition, specification of polar and stalk cells via germline-to-soma signaling involving Delta/Notch, is also necessary for proper egg chamber formation (Grammont and Irvine, 2001
; Lopez-Schier and St Johnston, 2001
). It is possible then that the correct timing of events in the mid-germarial region for proper encapsulation and egg chamber budding is achieved by two signaling sources, the terminal filament (Hh signaling) and mature 16-cell germline cysts (Egghead, Brainiac, Gurken/TGF-
, and Delta signaling). The integration of all of these signals by prefollicular cells would be necessary for these cells to go through their developmental program in the appropriate time frame, thus allowing synchronous germline cyst maturation and encapsulation by prefollicular cells.
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ACKNOWLEDGMENTS |
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