1 Laboratory of Genetics,
2 Department of Biochemistry,
3 Laboratory of Molecular Biology, and
4 Howard Hughes Medical Institute, University of Wisconsin-Madison, Madison, WI 53706-1544 USA
*Author for correspondence (e-mail: jekimble{at}facstaff.wisc.edu)
Accepted 23 October 2001
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SUMMARY |
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Key words: POP-1, C. elegans, Gonadogenesis, Axis formation, Wnt signaling
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INTRODUCTION |
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Gonadogenesis has been described in detail at the cellular level for both sexes [reviewed by Hubbard and Greenstein (Hubbard and Greenstein, 2000)]. The gonadal primordium contains two somatic gonadal precursor cells, Z1 and Z4 (Fig. 1A), which flank two germline precursor cells, Z2 and Z3 (not shown in Fig. 1). The first division of Z1 and Z4 establishes the proximal-distal (PD) axes of the organ. The hermaphrodite gonad will develop two ovo-testes, each with a PD axis; the male gonad will have a single testis, and therefore a single PD axis (Hirsh et al., 1976
; Kimble and Hirsh, 1979
). These PD axes are determined by the daughters of Z1 and Z4: after this first division the daughters with distal fates reside at the poles and the daughters with proximal fates are located centrally in both sexes (Fig. 1B). This arrangement persists in hermaphrodites throughout gonadogenesis. In males, however, the two proximal daughters migrate anteriorly and the anterior distal daughter is displaced posteriorly (Fig. 1C, left). The resultant structure (Fig. 1C, right) places the two proximal daughters at the anterior and the two distal daughters at the posterior end, transforming the symmetrical structure with two opposing PD axes into an asymmetrical structure with a single PD axis. In this way, the developing gonads acquire sex-specific polarities after a single division of Z1 and Z4.
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In addition to specification of leader cells, two other regulatory functions are assigned early in gonadogenesis. In both sexes, the Z1/Z4 distal daughters (or granddaughters) signal the germline to proliferate (Kimble and White, 1981). In hermaphrodites, the germline proliferation and leader functions reside in the same cell (the DTC), whereas in males, they are allocated to separate cells: germline control in the DTCs and leader function in the linker cell (LC). Another regulatory cell specified during early gonadogenesis is the anchor cell (AC), which is specific to hermaphrodites and arises from the proximal Z1/Z4 daughters (Fig. 1D). The two cells competent to become the AC use lateral signaling (arrows, Fig. 1D) to make one AC and one ventral uterine (VU) precursor cell (Kimble, 1981
). The AC induces vulval development in the ventral hypodermis (Kimble, 1981
) and also induces nearby uterine precursors to take on the
cell fate (Newman et al., 1995
).
Another key event, which completes early gonadogenesis, is formation of a somatic primordium; the blast cells in this primordium generate the somatic gonadal structures of the adult (Kimble and Hirsh, 1979). In hermaphrodites, all somatic gonadal cells, except the DTCs, migrate centrally and coalesce to create a hermaphrodite-specific somatic gonadal primordium (SPh) during the late L2 and early L3 stage (Fig. 1D). In males, all somatic gonadal precursor cells, except the DTCs, cluster anteriorly to form the male-specific somatic gonadal primordium in early L2 (SPm) (Fig. 1E). These sex-specific somatic primordia (SP) prefigure the shape and pattern of the adult somatic gonadal structures.
Several genes are critical for early gonadogenesis [reviewed by Hubbard and Greenstein (Hubbard and Greenstein, 2000)]. Of particular importance for this work are lin-17 (Sternberg and Horvitz, 1988
) and sys-1 (Miskowski et al., 2001
). Both lin-17 and sys-1 affect the asymmetric division of Z1 and Z4. In lin-17 nonsense mutants and sys-1 strong loss-of-function mutants, Z1 and Z4 can divide symmetrically and generate two daughters that adopt the same, proximal fate (Fig. 1F,G). This is the Sys phenotype, for symmetrical sisters (Miskowski et al., 2001
). The lin-17 gene encodes a frizzled-like receptor (Sawa et al., 1996
), implicating Wnt signaling in control of Z1/Z4 asymmetric divisions. The sys-1 gene encodes a novel protein, providing no additional clue to biochemical function (J. Miskowski, A. Kidd and J. K., unpublished). Although the sys-1 and lin-17 mutant phenotypes are similar, they are not identical (Miskowski et al., 2001
; Sternberg and Horvitz, 1988
). Whereas lin-17 null mutants have a low penetrant (
30%) Sys gonadal phenotype in both sexes, sys-1 is fully penetrant in hermaphrodites, but poorly penetrant (
30%) in males. In addition, lin-17 is involved in asymmetric divisions in many tissues; however, the post-embryonic effects of sys-1 appear to be limited to the gonad. Therefore, these two genes overlap functionally, but are also distinct.
In this work, we introduce the sys-2 locus. We find that sys-2 is allelic with pop-1, a TCF/LEF-1 transcription factor that activates genes in response to Wnt signaling (Lin et al., 1995). We therefore have dropped the sys-2 gene name, but retained the Sys name to describe Z1/Z4 division defects typical of sys-1, lin-17 and pop-1(Sys) mutants. The two pop-1(Sys) alleles are both missense mutations, one in the ß-catenin binding domain and one in the HMG box. The phenotypes of these two alleles are distinct, both from each other and from those of pop-1(RNAi) progeny. To explore the pathway controlling Z1/Z4 asymmetry, we analyzed components of the canonical Wnt signaling pathway and components of a Map kinase pathway that regulate POP-1 function. We find that animals lacking either the ß-catenin homologue wrm-1 or the nemo-like kinase (NLK) homologue lit-1 have typical Sys gonadal defects. Similarly, loss of lit-1 in a post-embryonic cell, called the T cell, also results in the same phenotype as loss of pop-1 (Herman, 2001
). These results contrast to what has been found in the C. elegans embryo and in vertebrates, where lit-1 opposes pop-1 function (Ishitani et al., 1999
; Kaletta et al., 1997
; Meneghini et al., 1999
; Rocheleau et al., 1999
).
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Materials and Methods |
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Isolation and genetic characterization of sys-2 mutations
Two pop-1 alleles were isolated in an F2 screen following mutagenesis with ethyl methane sulfonate (EMS). These two mutations failed to complement and mapped to the left arm of chromosome I between lin-17 and mek-2 by 3-factor and deficiency mapping. The deficiency tDf4 complemented pop-1(q645) and tDf3 failed to complement pop-1(q645). From pop-1/mek-2 unc-11, 18/18 Unc non-Mek progeny carried pop-1(Sys). We used the deletion allele lin-17(sy277) as a molecular marker for mapping. From pop-1 unc-11/ lin-17, 53/53 Unc non-Sys carried the lin-17 deletion. We also failed to separate pop-1(zu189) from pop-1(q645): from zu189/q645 unc-11, 46/46 Unc-non Sys were Mel.
pop-1(q624) is recessive: wild-type males were crossed into pop-1(q624) mec-8/hT2[qIs48]; all cross-progeny were wild type (n=91). pop-1(q645) shows minor dominance: wild-type males were crossed into pop-1(q645) mec-8/hT2[qIs48]; 1% of pop-1(q645)/+ cross progeny had one gonad arm (n=77). In addition, whole broods were scored from pop-1(q645)/+: two broods were scored at 25°C, and three at 20°C. At 25°C, 24% had no gonad arms, 2% had one gonad arm, and 72% had two gonad arms. At 20°C, 26% had no gonad arms and 73% had two gonad arms. At both temperatures about 1% of embryos were dead. Because pop-1(q624) can be L1 lethal, we scored total survivors from eggs laid during an 8 hour time period, rather than whole broods. From a heterozygous pop-1(q624)/+ parent, 6% arrested or died as L1, and from a homozygous pop-1(q624) parent 65% arrested or died as L1. Animals that did not arrest as L1 grew to adulthood; gonad arms were scored in survivors (Table 1). This scheme was also used to assay lethality for pop-1(q645)/tDf3 and pop-1(RNAi). To assay lethality in pop-1(q624)/tDf3, we crossed pop-1(q624)/hT2[qIs48] females (feminized by fog-1(RNAi)) with tDf3/hT2[qIs48] males. Fewer than one pop-1(q624)/tDf3 (non-green) survivor was seen per mother; gonad arms were scored in survivors (Table 1).
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Cell lineage and laser ablation
Cell lineages were examined by standard methods (Sulston and Horvitz, 1977). Laser ablations were done as described previously (Bargmann and Avery, 1995
) using a Micropoint Ablation Laser System (Photonics Instruments, Inc. Arlington, IL). pop-1(q645) homozygotes were obtained as non-green L1s from pop-1(q645)/hT2[qIs48] parents. Either Z2 or Z3 was ablated in these animals prior to lineage analysis to reduce complexity; this ablation does not affect the Z1/Z4 lineage. pop-1(RNAi) males were selected for lineage by presence of a large B cell. For Z1.a/Z4.p ablations and Z1.p/Z4.a ablations, cells were ablated soon after they were born. Ablations were verified by DIC 1-2 hours post-operative.
Mutant rescue and RNAi
To test for cosmid rescue, pop-1(q645) unc-11(e47)/hT2 hermaphrodites were injected with 9 ng/µl BF8 cosmid and 100 ng/µl pRF4 (Mello and Fire, 1995). Fertile Rol Uncs were found among the F2, and shown genetically to be homozygous for pop-1(q645).
pop-1 template DNA for double stranded RNAi synthesis was made by PCR from genomic DNA, using primers with T7 sites at both ends. There are no other genes in the C. elegans genome that could be targeted by this RNA. Template DNA for other Wnt pathway members (except bar-1 and mom-5, see below) was made by RT-PCR to the 5' end of the gene. bar-1 and mom-5 template was made by PCR from genomic DNA. PCR products were subcloned and amplified using primers with T7 promoter sites at the 5' ends. Double stranded RNA was produced using the MEGAscript T7 Kit (Ambion Inc.). All dsRNA products included at least 650 bp of exon sequence. RNA to each gene was injected into N2 and unc-32 rde-1 at both 2.5 and 1 mg/ml. Injected animals were crossed with N2 males or males carrying GFP reporters. We also injected lin-44(n1792) mutants with egl-20, cwn-1, or cwn-2 dsRNA, each at 1 mg/ml. In addition, we soaked lin-44(n1792) mutants for 2 days (with E. coli) in the following dsRNA combinations: mom-2 and egl-20; mom-2 and cwn-1; mom-2 and cwn-2. Each RNA was at 1 mg/ml in M9.
Molecular analysis
Exons of pop-1 were sequenced from q624 and q645 homozygotes. Template DNA for sequencing was made by amplifying pop-1 exons from homozygotes using ExpandTM High Fidelity PCR System (Boehringer Mannheim). At least three independent PCR reactions were sequenced from each mutant, and two independent RT-PCR reactions were sequenced from pop-1(q645) mutants. Big-Dye Terminator Ready Reaction Mix was used for sequencing reactions (PE/Applied BioSystems). Reactions were run by the Blattner Lab sequencing service, Department of Genetics, UW-Madison. Protein alignments were made using PILEUP from GCG Wisconsin Package v.10 (Genetic Computer Group, Madison, WI).
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RESULTS |
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Early gonadogenesis in pop-1(Sys) hermaphrodites
The pop-1(Sys) hermaphrodites exhibit typical Sys gonadal defects. First, whereas wild-type hermaphrodites have two DTCs (Fig. 3A), pop-1(q645) mutants have none (Fig. 3B, Table 1). Similarly, pop-1(q624) mutants can lack gonadal arms and DTCs (Table 1, not shown). Second, whereas wild-type hermaphrodites possess a single AC (Fig. 3D), pop-1(Sys) mutants often have two or sometimes 3 AC (Fig. 3E, Table 1). Third, whereas wild-type hermaphrodites assemble an SPh (Fig. 3A), this structure is never seen in pop-1(q645) hermaphrodites. Instead, a ring of somatic gonadal cells surrounds the germline at the L2/L3 stage (Fig. 3B, arrowheads).
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We next examined the early Z1/Z4 lineage in pop-1(q645) hermaphrodites (Fig. 4). Normally, Z1 and Z4 generate daughters with different fates (Fig. 4A). However, in pop-1(q645) mutants, Z1 and Z4 appear to generate daughters with equivalent fates (Fig. 4B). Although some variability was seen (see legend to Fig. 4), all Z1/Z4 daughters could divide twice, a pattern normally restricted to proximal daughters. Furthermore, all four daughters could produce AC/VU cells, as shown by laser ablation and assaying vulva formation. When Z1.p and Z4.a were ablated in pop-1(q645) hermaphrodites, a vulva was nearly always formed (9/10); similarly, when Z1.a and Z4.p were ablated, a vulva was made (6/6). However, when Z1 and Z4 were ablated, no vulva was formed (5/5). Therefore, the pop-1(Sys) Z1/Z4 daughters are equivalent with respect to their pattern of cell divisions and generation of AC/VU cells.
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In addition to the early Z1/Z4 Sys defect, pop-1(RNAi) males have another gonadal defect not seen in pop-1(Sys) mutants: the gonadal arm does not elongate, even though the LC is correctly specified, as assayed by normal morphology and expression of lag-2::GFP (Fig. 5E,F). This failure in gonadal elongation results in a severely malformed gonad. Furthermore, pop-1(RNAi) males usually die in L3 or L4 owing to tail defects (see below), making their analysis beyond L2 difficult.
Non-gonadal defects of pop-1(Sys) mutants and pop-1(RNAi) progeny
Both pop-1(Sys) mutants and pop-1(RNAi) progeny exhibit non-gonadal defects in addition to the gonadal defects described above. Most severe is L1 lethality, which is found among pop-1(q624) mutants and zygotic pop-1(RNAi) animals, but is rare or non-existent among pop-1(q645) progeny (Table 1). The dead L1s exhibit various defects, including a detached pharynx, misshapen body, and incorrect assembly of the gonadal primordium (not shown). Among pop-1(RNAi) survivors, most hermaphrodites develop to adulthood, whereas most males die during L3 or L4. Virtually all pop-1(RNAi) animals are uncoordinated, and nearly all males exhibit tail defects. pop-1(RNAi) and pop-1(Sys) hermaphrodites often have a protruding vulva, and fertile pop-1(q624) hermaphrodites are frequently egg-laying defective.
To monitor a non-gonadal defect that depends on Wnt signaling (Herman et al., 1995; Sawa et al., 1996
), we assayed T cell polarity in both pop-1(Sys) mutants and pop-1(RNAi) animals. In wild-type hermaphrodites, the posterior T cell daughters give rise to the phasmid socket cells and the anterior daughters give rise to primarily hypodermis (Sulston and Horvitz, 1977
). In the absence of Wnt signaling components, both daughters generate hypodermis and no phasmids are made (Herman, 2001
; Herman and Horvitz, 1994
; Herman et al., 1995
). We therefore scored phasmids in pop-1(Sys) mutants and pop-1(RNAi) animals using a dye-filling assay (Herman and Horvitz, 1994
). In both pop-1(Sys) mutants, fewer than normal phasmids were made, whereas in pop-1(RNAi) animals, almost none were found (Table 3). Therefore, both alleles affect T cell polarity in addition to Z1/Z4 polarity. Interestingly, the percentage of pop-1(Sys) mutants with T cell lineage defects was roughly equivalent to the percentage of pop-1(Sys) males with Z1/Z4 defects, both of which were substantially lower than the percentage of pop-1(Sys) hermaphrodites with Z1/Z4 defects (Table 3).
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A similar simple conclusion could not be made for pop-1(q645). This allele is fully penetrant for the Sys gonadal defect, as is pop-1(q645)/tDf3 (Table 1). However, in contrast to pop-1(q624)/tDf3 animals, which never made gonadal arms, a few q624/q645 hermaphrodites did possess gonadal arms (Table 1), suggesting that pop-1(q645) is a strong loss-of-function allele with respect to DTC production, but not a null. Intriguingly, L1 lethality was not seen in pop-1(q645) mutants and was far less severe in pop-1(q645)/tDf3 than pop-1(q624)/tDf3 animals (Table 1). The full penetrance of pop-1(q645) with respect to hermaphrodite gonadogenesis contrasts sharply with its extremely weak effect on L1 viability. We speculate that the pop-1(q645) mutation may affect a regulatory region essential for hermaphrodite gonadogenesis, but not for most other pop-1 functions (see Discussion).
L1 lethality was observed among pop-1(q624) mutants derived from a heterozygous mother (6%, n=144), but was more frequent among pop-1(q624) mutants derived from a homozygous mother (65%, n=147). Therefore, maternal pop-1 product plays a role that is crucial for L1 survival in addition to its previously known role in controlling early embryogenesis (Lin et al., 1995).
Wnt signaling and gonadogenesis
The pop-1 gene encodes a key transcription factor acting at the end of the Wnt pathway in C. elegans [reviewed by Wodarz and Nusse (Wodarz and Nusse, 1998)]. To determine what other Wnt signaling components might be involved in early gonadogenesis in nematodes, we used a combination of RNAi and available mutants to look for Sys defects. Table 4 summarizes our results. We detected no gonadogenesis defect for any of the five known Wnt homologues, by using RNAi for each of the five, or by analyzing mutants of three of them, or by double and triple RNAi (see Materials and Methods). However, 3% of animals mutant for the porcupine homologue, mom-1, had only one gonadal arm (n=72). Therefore, a Wnt ligand may be involved in Z1/Z4 polarity. We next examined three frizzled receptor homologues (Table 4). Previous work showed that a lin-17 nonsense mutant has a low penetrance Sys phenotype (Sternberg and Horvitz, 1988
). Using RNAi, we confirmed this effect. RNAi directed against either of the other two frizzled receptor homologues, mom-5 and cfz-1, did not yield Sys defects. In addition, mom-5 mutants do not show Sys defects. Therefore, LIN-17 is the only frizzled receptor known to function in the early gonadal lineage, and its role is not essential. In RNAi experiments, genes with known mutant phenotypes exhibited expected defects (for example, mom-2(RNAi) produced 100% dead eggs when wild-type animals were injected), suggesting that RNAi of these genes was working to some extent.
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DISCUSSION |
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During normal gonadogenesis, POP-1 governs the asymmetric division of Z1 and Z4, and thereby controls the gonadal PD axes and the generation of regulatory cells essential for subsequent morphogenesis. In the absence of POP-1 function, Z1 and Z4 generate equivalent daughters that both assume a proximal fate. Hermaphrodite gonads lacking pop-1 lose their PD axes and fail to generate regulatory cells required for gonad elongation and germline proliferation. Male gonads lacking pop-1 also lose their PD axis they have no cells with distal fates and therefore no distal end. However, the male gonad acquires an apparently normal polarity, which reflects the male-specific specification of an AP axis in this organ.
How might POP-1 govern Z1/Z4 asymmetry? We suggest two simple models (Fig. 6A), although they are not mutually exclusive and others certainly exist. Both models take advantage of the fact that Z1 and Z4 contact each other ventrally beneath the two germline precursor cells, Z2 and Z3 (F-H. Markussen, L. Mathies, Y. Li, and J. Kimble, unpublished). In the first model (Fig. 6A, left), a Wnt signal polarizes Z1 and Z4, which leads to enhanced POP-1 activity in the distal daughter. Polarization may result from an inhibitory signal in the underlying hypodermis or from a decreased access of the Wnt to proximal regions of Z1/Z4. In the second model (Fig. 6A, right), no Wnt signal is invoked. Instead, contact between Z1 and Z4 (or contact between Z1/Z4 and the hypodermis) polarizes the cell (for example, excluding LIN-17 from the proximal region), which leads to enhanced POP-1 activity in the distal daughters.
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Identification of two distinct pop-1(Sys) mutations
Prior to this paper, only one pop-1 mutation had been reported. This allele, pop-1(zu189), is a transposon insertion into the pop-1 3' untranslated region that abolishes maternal pop-1 mRNA, but leaves zygotic pop-1 mRNA intact (Lin et al., 1995; Morse and Bass, 1999
). The pop-1(zu189) allele identifies a regulatory site for maternal pop-1 mRNA, but does not shed light on regulatory regions within POP-1 protein itself. In this paper, we report two pop-1(Sys) mutations that change the pop-1 coding region and have dramatic effects on gonadogenesis. Our characterization of these alleles as well as zygotic pop-1(RNAi) suggests that one, pop-1(q624), is a typical partial loss-of-function mutation and that the other, pop-1(q645), is unusual. The pop-1(q624) defects are found at low penetrance, are similar to those observed by pop-1(RNAi) (e.g. L1 lethality, Sys gonads, T cell defects), and become more penetrant when the allele is placed over a deficiency. This mutation alters a conserved amino acid in the HMG box DNA binding domain which is conserved specifically in TCF/LEF-1 type HMG proteins (Laudet et al., 1993
), suggesting that the pop-1(q624) mutation may affect either recognition of the TCF/LEF-1 consensus sequence or DNA binding affinity, thereby lowering POP-1 activity.
Unlike the weak pop-1(q624) mutation, pop-1(q645) is fully penetrant for the Sys gonadal defect in hermaphrodites, but exhibits no L1 lethality. Therefore, pop-1(q645) alters a residue essential for hermaphrodite gonadogenesis, but not for other pop-1-dependent events. The pop-1(q645) mutation alters an aspartic acid to glutamic acid in the ß-catenin binding domain. This amino acid is conserved in all TCF/LEF-1 homologues and, through analysis of vertebrate homologues, has been shown to be essential for ß-catenin binding and for ß-catenin and TCF/LEF-1 to activate transcription of target genes (Graham et al., 2000; Hsu et al., 1998
; von Kries et al., 2000
). Although two missense mutations affecting the ß-catenin binding domain of the D. melanogaster TCF/LEF-1 homologue, Pan, have been isolated, neither of these two mutations affects residues conserved among all TCF/LEF-1 homologues (Brunner et al., 1997
). As the only mutation isolated thus far in a developmental system that changes a highly conserved amino acid in the ß-catenin binding domain, the pop-1(q645) missense mutation may shed new light on TCF/LEF-1 function during development. It is striking that the ß-catenin homologue critical for Z1/Z4 asymmetry is WRM-1, which does not bind the POP-1 ß-catenin binding domain (Korswagen et al., 2000
; Natarajan et al., 2001
; Rocheleau et al., 1999
). We speculate that the POP-1 ß-catenin binding site may interact with a regulator in Z1 and Z4 that differentially affects that tissue.
Z1/Z4 asymmetry, POP-1 control and sexual dimorphism?
Because pop-1(q645) mutant hermaphrodites are always sterile while mutant males can be fertile, we looked for sex-specific defects in pop-1(Sys) mutants and pop-1(RNAi) animals. We found that POP-1 controls Z1/Z4 asymmetry in both sexes. Unlike pop-1(RNAi), which has equivalent strong effects on both sexes, the two pop-1(Sys) mutations affect hermaphrodite gonadogenesis more strongly than male gonadogenesis (Table 3). This difference in the effect of pop-1 mutations may reflect a more stringent requirement for pop-1 activity in the hermaphrodite gonad, it may reflect a more stringent dependence of the hermaphrodite gonad on correctly establishing the PD axes, or it may reflect a sex-specific regulation of POP-1. If sex-specific regulation occurs, the unusual pop-1(q645) mutation may identify the POP-1 ß-catenin binding domain as the site of that regulation.
PD axis specification is required for SP formation in hermaphrodites, but not in males. In pop-1(Sys) and pop-1(RNAi) hermaphrodites, SPh formation is disrupted resulting in a disorganized organ and sterility. However, in pop-1(Sys) and pop-1(RNAi) males, early cell rearrangements that establish the AP axis of the male gonad occur as normal, and overall organ polarity appears normal. Therefore, AP axis specification in the male gonad does not require proper specification of the PD axis.
The POP-1 pathway controls Z1/Z4 asymmetry
We surveyed Wnt signaling components and additional regulators of POP-1 for control of Z1/Z4 asymmetry and found that a decrease in either WRM-1, a ß-catenin homologue, or LIT-1, a nemo-like kinase (NLK) homologue, led to Z1/Z4 defects similar to those of decreased POP-1 activity. Furthermore, previous work showed that the lin-17 receptor is involved, albeit with lower penetrance (Sawa et al., 1996; Sternberg and Horvitz, 1988
). Surprisingly, we identified no Wnt signal as critical for Z1/Z4 polarity. This negative result may mean that a Wnt signal is not required, that the signal is encoded by redundant wnt genes, or that it is not sensitive to RNAi. At present, we cannot distinguish among these possibilities. Our models (Fig. 6A) leave open the possibility that a Wnt signal may exist.
Fig. 6B summarizes the pathway of POP-1 control in the gonad and compares that control to what has been observed in other C. elegans tissues. In Z1/Z4, WRM-1 and LIT-1 are both required for POP-1 activity. All three genes are required for the distal fate. By contrast, WRM-1 and LIT-1 antagonize POP-1 activity in the embryo (Kaletta et al., 1997; Meneghini et al., 1999
; Rocheleau et al., 1999
) and LIT-1, but not WRM-1, is involved in controlling T cell polarity (Herman, 2001
; Rocheleau et al., 1999
).
We envision two explanations for how WRM-1 (a ß-catenin) and LIT-1 (NLK) may act to enhance POP-1 activity in the gonad. One simple explanation is that WRM-1 and LIT-1 may positively regulate POP-1; this idea is based on classical results that ß-catenins are TCF co-activators [reviewed by Wodarz and Nusse (Wodarz and Nusse, 1998)], and that NLK is complexed with TCF and ß-catenin (Ishitani et al., 1999
). The WRM-1 ß-catenin does not bind the POP-1 ß-catenin binding domain per se, but weakly binds full length POP-1 (Korswagen et al., 2000
; Natarajan et al., 2001
; Rocheleau et al., 1999
). Perhaps WRM-1 interacts with POP-1 in Z1/Z4 and serves there as a coactivator. Such a physical interaction might be stabilized by another binding protein, such as LIT-1, which is known to bind POP-1 (Natarajan et al., 2001
; Rocheleau et al., 1999
). A second possibility is that WRM-1 and LIT-1 negatively regulate POP-1, reducing its level to an active state; this rather counterintuitive model was proposed by Herman (Herman, 2001
) to explain how POP-1 might be regulated in the T cells. If the Herman model holds true in Z1/Z4 as well, then WRM-1/LIT-1 may downregulate POP-1 in the distal daughters and thereby bring POP-1 to the appropriate level to drive distal fates. The first model predicts that POP-1 will be more abundant in the distal daughters, whereas the Herman model predicts POP-1 to be more abundant in the proximal daughters. Unfortunately, POP-1 antibodies currently available do not reliably stain the L1 gonad, although hypodermal and other tissues stain well (K. Siegfried, unpublished). We have therefore been unable to distinguish between these two models.
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ACKNOWLEDGMENTS |
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REFERENCES |
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Bargmann, C. I. and Avery, L. (1995). Laser killing of cells in Caenorhabditis elegans. In Caenorhabditis elegans: Modern Biological Analysis of an Organism, (ed. H. F. Epstein and D. C. Shakes), pp. 225-250. San Diego: Academic Press, Inc.
Blelloch, R., Santa Anna-Arriola, S., Gao, D., Li, Y., Hodgkin, J. and Kimble, J. (1999). The gon-1 gene is required for gonadal morphogenesis in Caenorhabditis elegans. Dev. Biol. 216, 382-393.[Medline]
Brenner, S. (1974). The genetics of Caenorhabditis elegans. Genetics 77, 71-94.
Brunner, E., Peter, O., Schweizer, L. and Basler, K. (1997). pangolin encodes a Lef-1 homologue that acts downstream of Armadillo to transduce the Wingless signal in Drosophila. Nature 385, 829-833.[Medline]
Eisenmann, D. M. and Kim, S. K. (2000). Protruding vulva mutants identify novel loci and Wnt signaling factors that function during Caenorhabditis elegans vulva development. Genetics 156, 1097-1116.
Fire, A., Xu, S., Montgomery, M. K., Kostas, S. A., Driver, S. E. and Mello, C. C. (1998). Potent and specific genetic interference by double-stranded RNA in Caenorhabditis elegans. Nature 391, 806-811.[Medline]
Friedman, L., Santa Anna-Arriola, S., Hodgkin, J. and Kimble, J. (2000). gon-4, a cell lineage regulator required for gonadogenesis in Caenorhabditis elegans. Dev. Biol. 228, 350-362.[Medline]
Graham, T. A., Weaver, C., Mao, F., Kimelman, D. and Xu, W. (2000). Crystal structure of a ß-catenin/Tcf complex. Cell 103, 885-896.[Medline]
Greenwald, I. S., Sternberg, P. W. and Horvitz, H. R. (1983). The lin-12 locus specifies cell fates in Caenorhabditis elegans. Cell 34, 435-444.[Medline]
Herman, M. A. (2001). C. elegans POP-1/TCF functions in a canonical Wnt pathway that controls cell migration and in a noncanonical Wnt pathway that controls cell polarity. Development 128, 581-590.
Herman, M. A. and Horvitz, H. R. (1994). The Caenorhabditis elegans gene lin-44 controls the polarity of asymmetric cell divisions. Development 120, 1035-1047.
Herman, M. A., Vassilieva, L. L., Horvitz, H. R., Shaw, J. E. and Herman, R. K. (1995). The C. elegans gene lin-44, which controls the polarity of certain asymmetric cell divisions, encodes a Wnt protein and acts cell nonautonomously. Cell 83, 101-110.[Medline]
Hirsh, D., Oppenheim, D. and Klass, M. (1976). Development of the reproductive system of Caenorhabditis elegans. Dev. Biol. 49, 200-219.[Medline]
Hodgkin, J. (1997). Appendix 1. Genetics. In C. elegans II (ed. D. L. Riddle, T. Blumenthal, B. J. Meyer and J. R. Priess), pp. 881-1047. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory Press.
Hsu, S.-C., Galceran, J. and Grosschedl, R. (1998). Modulation of transcriptional regulation by LEF-1 in response to Wnt-1 signaling and association with ß-catenin. Mol. Cell. Biol. 18, 4807-4818.
Hubbard, E. J. A. and Greenstein, D. (2000). The Caenorhabditis elegans gonad: A test tube for cell and developmental biology. Dev. Dyn. 218, 2-22.[Medline]
Ishitani, T., Ninomiya-Tsuji, J., Nagai, S.-i., Nishita, M., Meneghini, M., Barker, N., Waterman, M., Bowerman, B., Clevers, H., Shibuya, H. et al. (1999). The TAK1-NLK-MAPK-related pathway antagonizes signalling between ß-catenin and transcription factor TCF. Nature 399, 798-802.[Medline]
Johnson, R. L. and Tabin, C. J. (1997). Molecular models for vertebrate limb development. Cell 90, 979-990.[Medline]
Kaletta, T., Schnabel, H. and Schnabel, R. (1997). Binary specification of the embryonic lineage in Caenorhabditis elegans. Nature 390, 294-298.[Medline]
Kimble, J. (1981). Alterations in cell lineage following laser ablation of cells in the somatic gonad of Caenorhabditis elegans. Dev. Biol. 87, 286-300.[Medline]
Kimble, J. and Hirsh, D. (1979). The postembryonic cell lineages of the hermaphrodite and male gonads in Caenorhabditis elegans. Dev. Biol. 70, 396-417.[Medline]
Kimble, J. E. and White, J. G. (1981). On the control of germ cell development in Caenorhabditis elegans. Dev. Biol. 81, 208-219.[Medline]
Korswagen, H. C., Herman, M. A. and Clevers, H. C. (2000). Distinct ß-catenins mediate adhesion and signalling functions in C. elegans. Nature 406, 527-532.[Medline]
Laudet, V., Shehelin, D. and Clevers, H. (1993). Ancestry and diversity of the HMG box superfamily. Nucleic Acids Res. 21, 2493-2501.[Abstract]
Lin, R., Thompson, S. and Priess, J. R. (1995). pop-1 encodes an HMG box protein required for the specification of a mesoderm precursor in early C. elegans embryos. Cell 83, 599-609.[Medline]
Maloof, J. N., Shangbo, J., Harris, J. M., Jongeward, G. D. and Kenyon, C. (1999). A Wnt signaling pathway controls Hox gene expression and neuroblast migration in C. elegans. Development 126, 37-49.
Mello, C. and Fire, A. (1995). DNA transformation. In Caenorhabditis elegans: Modern Biological Analysis of an Organism (ed. H. F. Epstein and D. C. Shakes), pp. 451-482. San Diego: Academic Press, Inc.
Meneghini, M. D., Ishitani, T., Carter, J. C., Hisamoto, N., Ninomiya-Tsuji, J., Thorpe, C. J., Hamill, D. R., Matsumoto, K. and Bowerman, B. (1999). MAP kinase and Wnt pathways converge to downregulate an HMG-domain repressor in Caenorhabditis elegans. Nature 399, 793-797.[Medline]
Miskowski, J., Li, Y. and Kimble, J. (2001). The sys-1 gene and sexual dimorphism during gonadogenesis in Caenorhabditis elegans. Dev. Biol. 230, 61-73.[Medline]
Morse, D. P. and Bass, B. L. (1999). Long RNA hairpins that contain inosine are present in Caenorhabditis elegans poly(A)+ RNA. Proc. Natl. Acad. Sci. USA 96, 6048-6053.
Natarajan, L., Witwer, N. E. and Eisenmann, D. M. (2001). The divergent Caenorhabditis elegans ß-catenin proteins BAR-1, WRM-1 and HMP-2 make distinct protein interactions but retain functional redundancy in vivo. Genetics 159, 159-172.
Newman, A. P., White, J. G. and Sternberg, P. W. (1995). The Caenorhabditis elegans lin-12 gene mediates induction of ventral uterine specialization by the anchor cell. Development 121, 263-271.
Pettitt, J., Wood, W. B. and Plasterk, R. H. A. (1996). cdh-3, a gene encoding a member of the cadherin superfamily, functions in epithelial cell morphogenesis in Caenorhabditis elegans. Development 122, 4149-4157.
Rocheleau, C. E., Downs, W. D., Lin, R., Wittmann, C., Bei, Y., Cha, Y.-H., Ali, M., Priess, J. R. and Mello, C. C. (1997). Wnt signaling and an APC-related gene specify endoderm in early C. elegans embryos. Cell 90, 707-716.[Medline]
Rocheleau, C. E., Yasuda, J., Shin, T. H., Lin, R., Sawa, H., Okano, H., Priess, J. R., Davis, R. J. and Mello, C. C. (1999). WRM-1 activates the LIT-1 protein kinase to transduce anterior/posterior polarity signals in C. elegans. Cell 97, 717-726.[Medline]
Roose, J. and Clevers, H. (1999). TCF transcription factors: molecular switches in carcinogenesis. Biochim. Biophys. Acta 97456, M23-M37.
Sawa, H., Lobel, L. and Horvitz, H. R. (1996). The Caenorhabditis elegans gene lin-17, which is required for certain asymmetric cell divisions, encodes a putative seven-transmembrane protein similar to the Drosophila Frizzled protein. Genes Dev. 10, 2189-2197.[Abstract]
Serrano, N. and OFarrell, P. H. (1997). Limb morphogenesis: connections between patterning and growth. Curr. Biol. 7, R186-R195.[Medline]
Seydoux, G. and Greenwald, I. (1989). Cell autonomy of lin-12 function in a cell fate decision in C. elegans. Cell 57, 1237-1245.[Medline]
Sokol, S. Y. (1999). Wnt signaling and dorso-ventral axis specification in vertebrates. Curr. Opin. Genet. Dev. 9, 405-410.[Medline]
Sternberg, P. W. and Horvitz, H. R. (1988). lin-17 mutations of Caenorhabditis elegans disrupt certain asymmetric cell divisions. Dev. Biol. 130, 67-73.[Medline]
Sulston, J. E. and Horvitz, H. R. (1977). Post-embryonic cell lineages of the nematode, Caenorhabditis elegans. Dev. Biol. 56, 110-156.[Medline]
Tabara, H., Sarkissian, M., Kelly, W. G., Fleenor, J., Grishok, A., Timmons, L., Fire, A. and Mello, C. C. (1999). The rde-1 gene, RNA interference, and transposon silencing in C. elegans. Cell 99, 123-132.[Medline]
Thorpe, C. J., Schlesinger, A., Carter, J. C. and Bowerman, B. (1997). Wnt signaling polarizes an early C. elegans blastomere to distinguish endoderm from mesoderm. Cell 90, 695-705.[Medline]
von Kries, J. P., Winbeck, G., Asbrand, C., Schwarz-Romond, T., Sochnikova, N., DellOro, A., Behrens, J. and Birchmeier, W. (2000). Hot spots in ß-catenin for interactions with LEF-1, conductin and APC. Nat. Struct. Biol. 7, 800-807.[Medline]
Whangbo, J., Harris, J. and Kenyon, C. (2000). Multiple levels of regulation specify the polarity of an asymmetric cell division in C. elegans. Development 127, 4587-4598.
Whangbo, J. and Kenyon, C. (1999). A Wnt signaling system that specifies two patterns of cell migration in C. elegans. Mol. Cell 4, 851-858.[Medline]
Wodarz, A. and Nusse, R. (1998). Mechanisms of Wnt signaling in development. Annu. Rev. Cell Dev. Biol. 14, 59-88.[Medline]