Cortical granule exocytosis in C. elegans is regulated by cell cycle components including separase

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First published online 3 October 2007
doi: 10.1242/dev.011361

Development 134, 3837-3848 (2007)
Published by The Company of Biologists 2007

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Cortical granule exocytosis in C. elegans is regulated by cell cycle components including separase

Joshua N. Bembenek¹^,*, Christopher T. Richie², Jayne M. Squirrell¹, Jay M. Campbell¹, Kevin W. Eliceiri¹, Dmitry Poteryaev³, Anne Spang³, Andy Golden² and John G. White¹

¹ University of Wisconsin-Madison, Laboratory of Molecular Biology, 1525 Linden Drive, Madison, WI 53706, USA.
² Laboratory of Biochemistry and Genetics, NIDDK, National Institutes of Health, Building 8, Room 323, 8 Center Drive, Bethesda, MD 20892-0840, USA.
³ Growth and Development, Biozentrum, University of Basel, Klingelbergstrasse 50/70, CH-4056 Basel, Switzerland.

^* Author for correspondence (e-mail: jbembenek{at}wisc.edu)

Accepted 13 August 2007

SUMMARY

TOP
SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In many organisms, cortical granules undergo exocytosis following fertilization,releasing cargo proteins that modify the extracellular covering ofthe zygote. We identified cortical granules in Caenorhabditis elegansand have found that degranulation occurs in a wave that initiates inthe vicinity of the meiotic spindle during anaphase I. Previousstudies identified genes that confer an embryonic osmotic sensitivityphenotype, thought to result from abnormal eggshell formation.Many of these genes are components of the cell cycle machinery.When we suppressed expression of several of these genes by RNAi,we observed that cortical granule trafficking was disruptedand the eggshell did not form properly. We conclude that osmotic sensitivityphenotypes occur because of defects in trafficking of cortical granulesand the subsequent formation of an impermeable eggshell. We identifiedseparase as a key cell cycle component that is required for degranulation.Separase localized to cortically located filamentous structures inprometaphase I upon oocyte maturation. After fertilization,separase disappeared from these structures and appeared on corticalgranules by anaphase I. RNAi of sep-1 inhibited degranulationin addition to causing extensive chromosomal segregation failures.Although the temperature-sensitive sep-1(e2406) allele exhibitedsimilar inhibition of degranulation, it had minimal effectson chromosome segregation. These observations lead us to speculatethat SEP-1 has two separable yet coordinated functions: to regulatecortical granule exocytosis and to mediate chromosome separation.

Key words: Anaphase promoting complex, Cortical granule exocytosis, Egg activation, Separase, Spindle assembly checkpoint, C. elegans, Meiosis

INTRODUCTION

TOP
SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Oocytes must coordinate specialized meiotic divisions with fertilization andthe subsequent transition to the mitotic program. Egg activationcomprises a sequence of events that occur in response to calciumtransients triggered by fertilization, including cortical granuleexocytosis and resumption of the cell cycle. Cortical granulesare large vesicles located at the cortex of mature oocytes ofmany species. Cortical granules secrete a collection of proteoglycansand enzymes that modify the extra embryonic covering of oocytes toprevent polyspermy (Wessel et al., 2001). At fertilization,inactivation of cytostatic factor, which arrests oocytes inmetaphase through inhibition of an E3 ubiquitin ligase knownas the anaphase-promoting complex/cyclosome (APC/C), allowsentry into anaphase and resumption of the cell cycle (Tunquistand Maller, 2003).

In the Caenorhabditis elegans gonad, oocytes arrested in prophase Iundergo maturation in response to signals from sperm and aresubsequently ovulated (Yamamoto et al., 2006). After fertilizationin the spermatheca, embryos pass into the uterus and extrudetwo polar bodies during consecutive meiotic divisions. Eggshellformation in nematodes occurs during meiosis (Chitwood and Chitwood,1974), such that the first polar body remains outside the permeabilitybarrier, whereas the second polar body does not (Polinko andStrome, 2000). The C. elegans eggshell consists of three layers,which we describe according to the following nomenclature: theoutermost vitelline layer present around the mature oocyte;a middle chitinous layer necessary for mechanical strength;and an internal lipid layer providing the permeability barrier (Rappleyeet al., 1999; Wharton, 1980). Although the process of eggshellformation in C. elegans is poorly understood, a recent genome-widescreen identified 109 genes likely to be required for eggshellformation (Sonnichsen et al., 2005), some of which are cellcycle regulatory components, suggesting a link between cellcycle regulation and eggshell formation.

Regulation of cell division requires faithful orchestrationof a wide diversity of cellular processes. During M-phase, preciseregulatory mechanisms ensure the fidelity of chromosome segregationand cell cleavage. During metaphase, a complex signaling pathwayknown as the spindle-assembly checkpoint (SAC) prevents entryinto anaphase before the correct alignment of chromosomes onthe metaphase plate (Musacchio and Salmon, 2007). The SAC preserveschromosome cohesion by inhibiting the APC/C (Peters, 2006).At the metaphase to anaphase transition, APC/C ubiquitinatessecurin, an inhibitory chaperone of the protease separase, leadingto its degradation by the proteasome (Nasmyth, 2002). Activeseparase then cleaves a subunit of the cohesin complex, allowingthe poleward movement of chromosomes during anaphase.

Inactivation of the C. elegans ortholog of separase, sep-1,causes chromosome nondisjunction, the osmotic integrity defectivephenotype (OID) and cytokinesis failures (Siomos et al., 2001).The osmotic integrity defective phenotype is also caused byinhibition of a number of cell cycle regulatory components (Sonnichsenet al., 2005), and has been suggested to be a non-specific consequenceof meiotic division failures. However, loss of other cell cyclegenes that cause severe meiotic defects does not give rise toan OID phenotype (Polinko and Strome, 2000), indicating thateggshell deposition is separable from cell division, although theseprocesses may be linked.

We have found that cortical granules form in developing oocytesand are exocytosed, leading to the formation of an impermeablethree-layered eggshell in C. elegans. The exocytosis of corticalgranules occurs during anaphase I and requires a number of cellcycle components, including separase. During anaphase I, separaselocalizes to cortical granules and may have a direct role inregulating cortical granule exocytosis. Our observations indicatethat events occurring during egg activation are coordinatedby cell cycle regulatory controls in C. elegans.

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Fig. 1. Identification of cortical granules. (A-C) Succynilated WGA-labeled cortical granules in C. elegans oocytes (A), and prometaphase I embryos (B), but not in embryos after meiosis I (C) (DNA in blue). (D-F) WGA-labeled cortical granules (D) are associated with SP12::GFP-labeled reticulate ER (E) at the cortex of a metaphase I embryo; merge in F. (G-I) UGTP-1::GFP-labeled 1 µm vesicles were clustered in prometaphase I (arrows, G) and redistributed across the cortex by metaphase I (arrows, H). Smaller cytoplasmic puncta remain after loss of the 1 µm vesicles (arrows, I). (J-L) WGA staining (J) co-localized with UGTP-1::GFP (K) in cortical granules in the cortex of a metaphase I embryo; merge in L. Scale bar: 10 µm.

	MATERIALS AND METHODS

TOP SUMMARY INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

C. elegans strains and alleles
The wild type was the Bristol strain N2, and all strains werecultured using standard techniques (Brenner, 1974

). Temperature-sensitivestrains were maintained at 16°C and shifted to 25°Cas L4 animals; all other strains were maintained at 20°C.The following strains were also used: WH0216 {sep-1(e2406) I/hT2[bli-4(e937)let-?(q782) qls48]}, WH0213 {sep-1(e2406) I; unc-119(ed3) III,ruls32 III[GFP::His-58 unc119(+)]/hT2[bli-4(e937) let-?(q782)qls48]}, HY604 mat-1(ye121) I, AZ212 {unc-119(ed3) III, ruls32 III[GFP::His-58unc119(+)]}, WH0327 {unc-119(ed3) III, ojIs23[GFP::SP12 unc119(+)]},WH0351 {unc-119(ed3) III, ojIs37[GFP::UGTP-1 unc119(+)]}, RT688{unc-119(ed3) III, pwIs281[GFP::CAV-1 unc119(+)]}, WH0416 {unc-119(ed3)III, ojIs58[SEP-1::GFP unc119(+)]}, WH0438 {unc-119(ed3) III, ojEx64[GFP::SEP-1unc119(+)]}.

Molecular biology
cDNA clones for syn-4 (yk493b10.3), cpg-1 (also known as cej-1- WormBase) (yk253a11) and cpg-2 (yk1687e03) were subclonedinto the L4440 vector for feeding RNAi (Kamath et al., 2001). Separasefeeding RNAi was performed as previously described (Siomos etal., 2001), and all other constructs were obtained from theAhringer library (Kamath et al., 2003). L4 animals were fedat 20°C for 24 hours (Fig. 4C-F), or as otherwise noted.The 2.5 kb ugtp-1 (ZK370.7) coding region was cloned from genomicDNA into the pID3.01 vector for biolistic transformation, asdescribed in (Poteryaev et al., 2005). The 5.2 kb coding sequenceof sep-1 was amplified from N2 genomic DNA using Phusion polymerase(NEB, Ipswich, MA, USA) and subcloned into the pJK derivativeplasmids of pFJ1.1 (Verbrugghe and White, 2004) that allow fordirectional cloning, and pie-1-driven expression of N- and C-terminalfusions with several worm-optimized fluorescent proteins includingmGFP (A206K mutant). Biolistic transformation was done as previouslydescribed (Praitis et al., 2001).

Immunohistochemistry and staining
The last 438 amino acids of the sep-1 open reading frame fusedto a hexa-histidine tag expressed in bacteria was purified usingthe Probond protein purification kit as per the manufacturer'sprotocol (Invitrogen, Carlsbad, CA, USA) under denaturing conditionsin 8 M urea. This purified protein was concentrated, dialyzedand used to raise rabbit polyclonal antibodies following standardprotocols (Covance Research Products, Berkeley, CA, USA). Theresulting immune serum was affinity-purified against antigen thathad been gel-purified and immobilized on nitrocellulose paper.Embryo staining was performed as described in Gonczy et al. (Gonczyet al., 1999) to preserve membrane structures. The followingdilutions, in PBS+0.05% BSA, were used: ${alpha}$ -SEP-1 antibodies, 1:200; ${alpha}$ -HIM-10 antibodies, 1:50; rhodamine-lectins from Vector Laboratories,1:10; tubulin antibody DM1 ${alpha}$ (Sigma, St Louis, MO, USA), 1:100;Alexa-conjugated secondary antibodies (Invitrogen), 1:200; andTO-PRO-3 Iodide (Invitrogen), 1:500. FM2-10 (Invitrogen) wasused at 17 µM, FM4-64 was used at 0.02 mg/ml and a fluorescein-conjugated3000-MW dextran (Invitrogen) was used at 0.5 mg/ml in blastomereculture medium (Shelton and Bowerman, 1996).

Microscopy
Mounting embryos
OID embryos were mounted in blastomere culture media (Sheltonand Bowerman, 1996) by hanging drop to relieve osmotic and mechanicalpressures. A toxicity effect (Siomos et al., 2001) was avoidedby removing bacteria and the mother carcass. Wild-type meiosisI embryos develop to hatching in these mounting conditions.

TEM
Animals were prepared for TEM as described previously (Poteryaevet al., 2005), without gluteraldehyde fixation and also imagedwith a Phillips CM 120 (FEI, Hillsboro, OR) at 80 kV, with aSoft Imaging Systems (Lakewood, CO) CCD camera and software,and a Tecnai T12 (FEI, Hillsborough, OR, USA) at 80 kV, withan ES500W CCD camera and software from Gatan (Pleasanton, CA,USA).

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Fig. 2. TEM of cortical granules. (A) A mature C. elegans oocyte contains cortical granules (arrows); inset shows higher magnification of vesicles near the oocyte chromosomes (asterisks). (B) An embryo within the spermatheca contains a cortical granule near the plasma membrane (upper right arrow), and a cluster of heterogeneous vesicles (lower arrows). (C) A metaphase I embryo contains cortical granules (arrows) distributed across the cortex (asterisk denotes chromosome in spindle). The cortical granules are found in close association with reticulate ER (A-C). (D) Embryo at metaphase II (chromosome in spindle indicated by white asterisk) lacks cortical granules, and the polar body (black asterisk) is trapped between eggshell layers (arrows). Scale bar: 2 µm.

Live cell imaging
Multiphoton laser-scanning microscopy (MPLSM) was done at LOCI (http://www.loci.wisc.edu) witha custom-designed multiphoton laser scanning optical workstation (Wokosinet al., 2003

). This system uses a Nikon Eclipse TE300 invertedmicroscope with a Nikon VC 60X Plan Apo oil-immersion lens (NA1.2) and 5W mode-locked Ti:sapphire laser (Spectra-Physics-Millennium/Tsunami)with excitation at 890 nm. The intensity data were collectedby a H7422 PMT (Hamamatsu) and the transmitted signal was collectedby a transmitted photodiode detector (Bio-Rad, Hercules, CA,USA). Image acquisition was done with WiscScan (http://www.loci.wisc.edu/wiscscan/). ASwept Field Confocal system (Prairie Technologies Inc, Middleton,WI, USA) with 488, 514 and 568 nm excitation lines was utilizedwith a Nikon Eclipse TE300 Microscope, 100x Superfluor LensNA 1.4 (Nikon, Melville NY) and a Dual-View beam splitter (RoperScientific, Tucson, AZ, USA) utilizing a FITC/Texas Red emissionset. Fixed samples were imaged using a Bio-Rad MRC 1024 confocalmicroscope (Hercules, CA, USA). To quantify degranulation, MPLSM wasdone with similar settings (which preserve embryo viabilityfor over 2000 scans) and vesicle fusion events were manuallycounted. Images were analyzed in ImageJ v1.37p (Abramoff etal., 2004

), and results were recounted on several data setsusing the point picker plugin. Images were processed in Photoshopv8.0 (Adobe Systems) using Gaussian blur to reduce noise, andlevels and curves to enhance contrast of the object of interest.

Statistics
Statistical calculations of mean, standard deviation and P-value weredetermined by fitting a one-way ANOVA model with SAS 9.1.3 on measurementsgathered from individual embryos.

RESULTS

TOP
SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of cortical granules
Cortical granules in oocytes of other organisms readily stainwith lectins (Hoodbhoy and Talbot, 2001), which bind sugar moleculesof glycosylated proteins. To obtain evidence that C. elegansoocytes contain cortical granules, we stained them with a panelof fluorescent-labeled lectins. Several lectins stained thevitelline layer, cytoplasmic vesicles and 1 µm vesiclesat the cortex of oocytes and embryos in meiosis I (see Fig.S1A-F in the supplementary material). Wheat germ agglutanin(WGA), used to identify cortical granules in human oocytes (Taleviet al., 1997), labeled 1 µm vesicles in C. elegans oocytesand meiosis I embryos, but not in older embryos (Fig. 1A-C). Eggshelllabeling with WGA appeared brighter in older embryos, suggestingthat it recognized a glycoprotein cargo of cortical granulesthat incorporates into the eggshell. The endoplasmic reticulum(ER) reorganizes into a reticulate structure in the cortex aroundthe time of fertilization (Poteryaev et al., 2005). We foundthat domains of the reticulate ER were closely associated withcortical granules in clusters during prometaphase I (see Fig.S1G-I in the supplementary material) that were redistributedevenly across the cortex during metaphase I (Fig. 1D-F). Therefore,we conclude that C. elegans contains cortical granules thatundergo dynamic trafficking similar to that of other organisms (Sardetet al., 2002).

We generated transgenic animals expressing a GFP fusion withZK370.7: a protein with sequence homology to transmembrane nucleotide-sugartransporters, predicted to transport UDP-galactose. This putativeGolgi marker (hereafter referred to as UGTP-1::GFP) labeledcytoplasmic puncta and large 1 µm vesicles in oocytesand young embryos, which were present for a narrow time windowafter fertilization. These vesicles were clustered in early prometaphaseI, redistributed within the cortex and lost by the end of meiosis I(Fig. 1G-I). We found that UGTP-1::GFP co-localized with WGA-stainedvesicles (Fig. 1J-L), indicating that it is packaged into corticalgranules. The observation that cortical granules contain UGTP-1::GFPsuggests that they may be Golgi-derived. CAV-1::GFP, a GFP fusionto caveolin, was previously shown to undergo trafficking consistent withcortical granule exocytosis (Sato et al., 2006), and also localizesto WGA-stained cortical granules more specifically than UGTP-1::GFP(see Fig. S1J-L in the supplementary material). Therefore, UGTP-1::GFPand CAV-1::GFP are convenient markers for live cell imagingof cortical granule trafficking.

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Fig. 3. A wave of exocytosis during anaphase I. C. elegans embryos expressing histone::GFP and labeled with the plasma membrane dye FM2-10 were imaged using SFC every 200 milliseconds. After the chromosome separation initiated (A), exocytic events (arrows) occurred near the spindle (B) and spread across the cortex (C,D) before the completion of anaphase I. Images in C and D are maximum projection summations of several frames in which a vesicle fusion event occurs. A gap is formed between the plasma membrane and the vitelline layer near the polar body (E, bracket). (F) Images of the plasma membrane before and after exocytosis, labeled with FM2-10 or a fluorescent dextran. Scale bar: 10 µm.

We used transmission electron microscopy (TEM) and observeda unique population of vesicles present in oocytes. Oocytesare fertilized approximately every 23 minutes (McCarter et al.,1999

), so that the age of each embryo can be inferred by itsposition within the uterus (see Fig. 4A). A mature oocyte containeda large number of vesicles closely associated with the reticulatedER (Fig. 2A). These approximately 1 µm vesicles had anunusual morphology reminiscent of the `refringent granules'shown to contribute to eggshell formation in other nematodespecies (Foor, 1967

). Prometaphase I embryos contained reticulateER interlaced with clusters of heterogeneous vesicles near thecortex (Fig. 2B). Metaphase I embryos contained the 1 µmvesicles dispersed throughout the cortex in close associationwith ER (Fig. 2C). These results are similar to our observationswith lectin staining. We were unable to capture an embryo duringdegranulation, but we anticipate that the vesicles dock at the plasmamembrane and are subsequently exocytosed based on our observationswith the light microscope (see below). Consistent with thisinterpretation, embryos at meiosis II or older did not containthe 1 µm vesicles (Fig. 2D). These observations suggestthat the 1 µm vesicles are cortical granules and thatthey may contribute to eggshell formation.

Cortical granule exocytosis occurs during anaphase I
In attempt to observe the rapid process of degranulation, weimaged embryos using swept field confocal (SFC) microscopy (PrairieTechnologies, Middleton, WI, USA) to acquire images every 200milliseconds. Embryos expressing histone::GFP (Praitis et al., 2001)were mounted with optimized techniques to preserve viability (seeMaterials and methods), labeled with the plasma membrane dyeFM2-10 and imaged by SFC (Fig. 3; see Movie 1 in the supplementary material).Interestingly, exocytosis began shortly after the homologouschromosomes separated during anaphase I in the region near themeiotic spindle (Fig. 3B). Fused vesicles incorporated FM2-10and appeared as pockets outlined with fluorescence. As anaphaseI proceeded, a wave of exocytosis spread across the cortex (Fig. 3B-D,F),and a gap opened between the vitelline layer and the plasmamembrane near the polar body (Fig. 3E). The size of the vesiclecavity ranged from 0.2 to 1.5 µm, consistent with thesize of cortical granules we observed by lectin staining andTEM.

To analyze secretion, we developed a correlative imaging techniqueusing MPLSM. We simultaneously acquired transmitted bright-fieldand fluorescence images by MPLSM. Embryos labeled with eitherFM2-10 or a fluorescent dextran dissolved in the culture mediumindicated vesicle-fusion events in the fluorescent image (Fig. 3F), whichappeared coincident with cup-shaped plasma membrane invaginationsin the bright-field image (see Movies 2 and 3 in the supplementary material).These observations demonstrate that the focal perturbationsof the plasma membrane visualized in the bright-field imagecorrelate with secretory events observed with plasma membraneand extracellular media labels and can serve as a marker forexocytosis.

To determine whether the wave of secretion during anaphase Irepresented the exocytosis of cortical granules, we observedthe loss of UGTP-1::GFP-labeled vesicles using correlative MPLSMimaging. Loss of UGTP-1::GFP-labeled vesicles coincided withthe appearance of plasma membrane perturbations visible in thebright-field image (see Movie 4 in the supplementary material).We also observed the loss of UGTP-1::GFP-labeled vesicles inthe presence of extracellular fluorescent dextran (see Movie5 in the supplementary material). In this experiment the signalof the extracellular dextran was saturating, whereas the UGTP-1::GFPsignal was significantly weaker. Therefore, the exchange ofvesicle contents with extracellular buffer after exocytosisresulted in a dramatic increase in fluorescence in the fusedvesicle cavity. We also imaged the fusion of CAV-1::GFP-labeledvesicles to the plasma membrane in the presence of the plasmamembrane dye FM4-64. The fluorescent signal from CAV-1::GFPis bright enough to image using SFC and capture two channelssimultaneously. FM4-64 photobleached quickly and caused a toxicityeffect when imaged by SFC with the 488 nm laser (not observedwith FM2-10, data not shown), but allowed us to capture shortmovies. After fusion, the vesicle cavity was immediately labeled withFM4-64 and co-localized with CAV-1::GFP, which remained on the cytoplasmicside of the plasma membrane (see Movie 6 in the supplementary material).These results demonstrate that cortical granule exocytosis occurs duringanaphase I.

OID proteins regulate cortical granules
Cortical granule exocytosis is required for the developmentof a polyspermy barrier on oocytes of other species (Wesselet al., 2001), therefore we hypothesized that it may contributeto formation of the eggshell in C. elegans. Inactivation ofgenes that lead to eggshell permeability cause the OID phenotype (Kaitnaet al., 2002; Rappleye et al., 1999; Siomos et al., 2001). Manyof the OID genes encode proteins either known or predicted tobe involved in protein trafficking through the ER and Golgi.A number of cell cycle regulators also give rise to OID whendepleted from the embryo. To gain further insight into the mechanismsthat regulate cortical granule exocytosis and determine if thisprocess is involved in eggshell formation, we assessed the fateof cortical granules following RNAi depletion of a selectionof OID genes representing these functional categories. Eachgene was tested in both the UGTP-1::GFP and CAV-1::GFP transgeniclines (see Table 1).

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Table 1. RNAi of OID genes disrupts cortical granule trafficking

Our results are consistent with the hypothesis that secretionof cortical granule proteoglycan cargo is required for eggshellformation. Previous results showed that depletion of SAR-1 (ZK180.4- WormBase), a small GTPase required for anterograde transportfrom the ER, prevented formation of cortical granules (Satoet al., 2006

). The syntaxin SYN-4 is required for vesicle fusionand is needed for eggshell formation and cytokinesis (Jantsch-Plungerand Glotzer, 1999

). syn-4(RNAi) oocytes had abnormal populationsof vesicles, sometimes accumulated at the plasma membrane (seeFig. S2E,F in the supplementary material). Eggshell chitin isgenerated by the chitin synthase, CHS-1 (Zhang et al., 2005

),a putative cargo protein. Oocytes and embryos in chs-1(RNAi)animals showed no obvious change in cortical granule trafficking (Fig. 3C).Depletion of the redundant CPG-1 and CPG-2 chitin-binding chondroitinproteoglycans, also putative cargo proteins, and the glycosylationenzyme, SQV-4, reduced the size, but not the trafficking ofcortical granules (see Fig. S2J,K in the supplementary material).CPG-1/-2 and SQV-4 may therefore be required to generate a significantmass of the proteoglycan cargo (the protein core and glycosylside chains, respectively) secreted through cortical granule exocytosisfor deposition of the eggshell.

The finding that membrane-trafficking regulators, but not putativecargo proteins, were required for cortical granule traffickingwas not surprising. However, it was less clear how cell cycleregulatory genes might affect cortical granules. Therefore,we tested the effect of RNAi-depletion of several cell cycleOID proteins on cortical granule trafficking. First, we analyzedregulators that control the overall timing of cell division. PrecociousCDK-1 activation occurs with wee-1.3(RNAi), resulting in prematureoocyte maturation (Burrows et al., 2006). wee-1.3(RNAi) oocyteshad large aggregates of UGTP-1::GFP-labeled puncta in the cytoplasm,which obscured the cortical granule population (see Fig. S2Ain the supplementary material). CAV-1::GFP appeared normal inoocytes depleted in WEE-1.3, although in some cases vesiclesmoved to the cortex prematurely (see Fig. S2B in the supplementary material).Timely entry into mitosis requires the active CDK complex. Depletionof the primary M-phase CDK, CDK-1, caused retention of cortical granulesin arrested embryos (see Fig. S2H in the supplementary material).To test the specificity of these effects, we depleted the CDKCKS-1 subunit by RNAi, which causes cytokinesis failures anddelayed exit from mitosis, but not OID (Polinko and Strome, 2000).As expected, cortical granule trafficking appeared normal incks-1(RNAi) embryos (see Fig. S2L in the supplementary material). Thesedata indicate that only a subset of genes that regulate globalcell cycle progression impact the trafficking of cortical granules.

A striking correlation exists between inhibiting genes thatregulate progress through the metaphase to anaphase transitionand the OID phenotype. czw-1 is homologous to the ZW10 spindleassembly checkpoint component (Karess, 2005), implicated in regulationof vesicle trafficking (Hirose et al., 2004). czw-1(RNAi) causedUGTP-1::GFP to localize in enlarged puncta and smaller cytoplasmicvesicles (see Fig. S2C in the supplementary material). CAV-1::GFPwas observed in small cytoplasmic vesicles (see Fig. S2D inthe supplementary material), indicating that CZW-1 may regulatebiogenesis of cortical granules. RNAi of APC/C subunits leadsto cell cycle arrest in metaphase I (Shakes et al., 2003) andcauses retention of CAV-1::GFP-labeled vesicles (Sato et al.,2006). We noticed that apc-2(RNAi) embryos retained clustersof cortical granules, reminiscent of wild-type prometaphaseI embryos (Fig. 4D). The RNAi depletion of the cyk-3 deubiquitinationenzyme causes OID and cytokinesis failures (Kaitna et al., 2002),and might disrupt ubiquitin-mediated regulation of the cell cycleor membrane trafficking. cyk-3(RNAi) embryos retained clusters ofcortical granules, similar to apc-2(RNAi) (see Fig. S2G in the supplementary material).These results suggest that the redistribution of cortical granulesthroughout the cortex is an ubiquitin-regulated process linkedto the cell cycle and that regulators of the metaphase to anaphase transitionalso control trafficking of cortical granules.

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Fig. 4. RNAi of OID genes affects cortical granules. (A) Organization of the C. elegans gonad, showing approximate cell cycle stages based upon the position of oocytes and embryos in wild-type animals. (B-D) Cortical granules labeled with UGTP-1::GFP (indicated by arrows; insets show higher magnification of vesicles). In wild-type animals, embryo +1 was undergoing meiosis I and contains cortical granules, whereas embryo +2 was in the first mitotic division and lacks cortical granules. (C) chs-1(RNAi) oocytes and embryos showed the same UGTP-1::GFP pattern as the wild type. (D) apc-2(RNAi) caused retention of clustered UGTP-1::GFP-labeled cortical granules. (E) sep-1(RNAi) caused retention of UGTP-1::GFP-labeled cortical granules in the first three embryos. Scale bar: 10 µm.

To gain further insight into the cell-cycle regulation of degranulation,we investigated the role of an important downstream effectorof APC/C in cortical granule exocytosis: separase. Inactivationof separase causes cytokinesis failures and delayed progressionthrough mitosis, similar to cks-1 (also known as dom-6 - WormBase).However, in contrast to cks-1, separase inactivation also causesOID. Consistent with this phenotype, we found that corticalgranules were retained in older embryos after depletion of separase(SEP-1) (Fig. 4E) or its inhibitory chaperone, securin (IFY-1)(see Fig. S2I in the supplementary material). To pursue theseobservations further, we examined embryos from an APC/C mutant[mat-1(ye121)] and from sep-1(RNAi) animals by TEM. APC/C mutantembryos were arrested in a meiotic state and contained corticalgranules (Fig. 5A). sep-1(RNAi) embryos were not arrested butstill retained cortical granules (Fig. 5B).

We compared the ultrastructure of the eggshell in wild-type,APC/C mutant and sep-1(RNAi) embryos. In the wild type, oocyteslacked an obvious covering (data not shown), but embryos inmeiosis I contained cortical granules and had a single coveringthat is likely to be the raised vitelline layer (Fig. 5C). Inolder embryos without cortical granules (i.e. putative post-degranulation),a three-layered eggshell was observed (Fig. 5D), similar toprevious results (Rappleye et al., 1999). APC/C mutant (Fig. 5E)and sep-1(RNAi) embryos (Fig. 5F) only had a single covering,similar to immature wild-type eggshells. Therefore, the formationof an impermeable three-layered eggshell requires secretionof cortical granule cargo, a process that is regulated by APC/C,separase and probably other OID genes.

sep-1 mutations and RNAi impair cortical granule exocytosis
The observation that inactivation of a subset of cell cycleregulatory genes caused the retention of cortical granules suggeststhat a specific regulatory pathway controls their exocytosis.Separase stood out among these genes because it is an importantregulator of anaphase, the time when degranulation occurs. Toinvestigate whether separase regulates degranulation, we measuredthe extent and kinetics of exocytosis during anaphase I. We monitoredthe progress of anaphase I by measuring the rate of homologous chromosomeseparation and counted the number of exocytic events observedin a single focal plane of histone::GFP expressing embryos labeledwith FM2-10. In wild-type embryos, secretion begins 92±8seconds (n=5 embryos) after the chromosomes initiate separationat 20°C, and 72±9 seconds (n=7 embryos) at 25°C.The exocytic wave occurs during the middle of anaphase beforethe polar body is extruded (Fig. 6C-E), and takes 121±6seconds to complete (n=7 embryos) at 20°C, and 76±10seconds (n=7 embryos) at 25°C. We observed 57±7 (n=7embryos), and 59±7 (n=10 embryos) exocytic events duringanaphase I at 20°C and 25°C, respectively (Fig. 6A,B).

We next analyzed the dynamics of degranulation in sep-1(RNAi)and sep-1(e2406) mutant embryos. Animals fed sep-1(RNAi) for17 to 20 hours at 25°C displayed chromosome nondisjunctionand dramatically delayed anaphase completion (Fig. 6B,F-H),consistent with sep-1 playing a role in CDK inhibition as observedin other species (Gorr et al., 2006). In addition, exocytosiswas significantly reduced (34±7 events, P<10^-4, n=9embryos, Fig. 6A,B), the anaphase spindle was disorganized andpolar body extrusion failed (Fig. 6F-H). Surprisingly, sep-1(e2406)embryos entered anaphase without severe chromosome nondisjunctionafter 12 to 14 hours at 25°C (Fig. 6B), but only 26±6 exocyticevents were observed (P<10^-4, n=9 embryos) (Fig. 6A,B). The reducedchromosome separation observed in sep-1(e2406) embryos during lateanaphase (Fig. 6I,J) may be due to steric hindrance of polarbody extrusion by the limited gap between the vitelline andplasma membrane and by the mislocalization of separase (see below).In some sep-1(e2406) embryos, a furrow enclosed the chromosomesat the cortex despite the reduced gap (Fig. 6K). In summary,both sep-1(RNAi) and sep-1(e2406) embryos have a similar reductionof cortical granule exocytosis, but sep-1(RNAi) shows much strongercell cycle delays, more severe chromosome nondisjunction, spindleand polar body extrusion defects. Therefore, sep-1(e2406) isa hypomorphic allele that is compromised for a subset of themultiple distinct functions of separase.

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Fig. 5. TEM of APC/C mutant and sep-1(RNAi) embryos. (A) The +2 embryo in a mat-1(ye121) C. elegans did not exit meiosis (asterisk indicates chromosomes in meiotic spindle) and retained cortical granules (arrows). (B) sep-1(RNAi) embryos were not arrested, but retained cortical granules (arrows). (C,D) Comparison of eggshell structures. In wild-type meiosis I embryos that contain cortical granules, a single vitelline layer was present (C). In mitotic embryos, cortical granules were lost and a three-layer eggshell (arrows) structure was observed (D). The +2 embryo in APC/C mutant (E) and sep-1(RNAi) (F) animals contained cortical granules and had a single vitelline layer (arrows), similar to immature wild-type eggshells. Scale bars: 3 µm in A,B; 0.5 µm in C-F.

As a control, we measured cortical granule exocytosis duringanaphase in cks-1(RNAi) embryos, which have cell cycle delaysand cytokinesis failures similar to those of separase mutants,but are not OID. We also analyzed chs-1(RNAi) embryos, whichare OID because they lack chitin in the eggshell (Zhang et al., 2005

).In both cases degranulation occurred normally (Fig. 6A). Thespindle of cks-1(RNAi) embryos did not undergo the normal rotationand movement observed in the wild type (Yang et al., 2005

),the distance that chromosomes separated during anaphase was reduced,and polar body extrusion failed (data not shown). However, after chromosomesseparated, a normal wave of cortical granule exocytosis occurred (58±8events, n=5 embryos, Fig. 6A). chs-1(RNAi) embryos failed polarbody extrusion, but cortical granule exocytosis occurred normally(56±8 events, n=3 embryos, Fig. 6A). The plasma membrane becamedeformed immediately after secretion (data not shown), possiblydue to the improper organization of eggshell components in theabsence of chitin. Together, these results demonstrate thatanaphase failures do not universally inhibit degranulation andthat not all OID phenotypes result from secretion failures.The observation that sep-1(e2406) embryos have relatively normalanaphase progression yet reduced cortical granule exocytosissuggests that separase may have a direct role in regulatingthis process.

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Fig. 6. The dynamics of the exocytic wave during anaphase I. C. elegans embryos labeled with histone::GFP and FM2-10 were imaged every 333 milliseconds using MPLSM. (A) Total exocytic events observed in wild-type, chs-1(RNAi) and cks-1(RNAi) embryos were nearly twice that of sep-1(e2406) and sep-1(RNAi) embryos. (B) Kinetic profiles of chromosome separation (plotted as a line) and exocytic events (columns) from single embryo recordings representative of average dynamics. Images from the movies are shown in C-K; brackets indicate distance measured between chromosomes, arrows indicate quantitated exocytic events. In wild type (green), degranulation initiated after chromosomes separated by 1.5 µm, and completed before polar body extrusion. In sep-1(RNAi) (red), chromosome separation was severely reduced, the wave of exocytosis was reduced and took much longer. By contrast, in sep-1(e2406) embryos (blue) chromosomes initially separated normally, but still had a reduced level of exocytosis that began after chromosomes separated by 2.5 µm. Scale bar: 10 µm.

Separase localizes to cortical granules during anaphase I
To examine further the role of separase in cortical granuleexocytosis, we determined the localization of separase by expressingGFP::SEP-1 in oocytes and young embryos (Fig. 7A-F and see Movie7 in the supplementary material) and by immunofluorescence with polyclonalantibodies directed against endogenous separase (Fig. 7G-I).During oocyte maturation, cytoplasmic separase rapidly accumulatedin the nucleus on homologous chromosomes. Separase also localizedto unusual filaments distributed throughout the cortex (Fig. 7A,B,H).Several proteins have been found in similar filaments in meiosisI embryos (Monen et al., 2005

), and also in Drosophila oocytes (Gillilandet al., 2007

). We found that separase co-localized in filamentswith HIM-10 (Fig. 8A-C), the homologue of the kinetochore componentnuf2 (Howe et al., 2001

). Before anaphase onset, separase waslost from these filamentous structures and accumulated on corticalvesicles (Fig. 7C,G). Separase co-localized with WGA-labeledcortical granules during anaphase I (Fig. 8D-F). Separase-labeled vesicleswere lost during anaphase I, beginning in the region near themeiotic spindle (Fig. 7G). We demonstrated that these vesiclesundergo exocytosis by live cell imaging with correlative MPLSMand double-labeling with fluorescent dextran (see Movies 8 and9 in the supplementary material). In mitotic embryos, separaselocalized to centrosomes, chromosomes and a diffuse cloud aroundthe metaphase plate and anaphase spindle (Fig. 7E,F,I).

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Fig. 7. Separase localizes to cortical granules in C. elegans. (A) Before ovulation, cytoplasmic GFP::SEP-1 rapidly accumulated in the nucleus, on chromosomes (asterisks) and cortical filaments (arrows). By metaphase I, GFP::SEP-1 was lost from filaments and appeared on cortical granules (B,C, arrows). GFP::SEP-1 disappeared during the exocytic wave in anaphase I and accumulated on the cortex near the polar body (D, arrow). (E,F) During mitosis, SEP-1::GFP localized to centrosomes (arrows), chromosomes (asterisks) and a diffuse cloud around the spindle. (G-I) Immunofluorescence with ${alpha}$ -SEP-1 (green) and DNA (blue). (G) Separase-labeled vesicles (arrows) were absent from the vicinity of the spindle in an embryo that had partly completed the exocytic wave during anaphase I (maximum projection image). Separase localizes to six central spindle elements (arrowhead) between homologous chromosomes and accumulates on the cortex near the polar body (asterisk indicates sperm pronucleus). (H) During prometaphase I, separase localized to filaments in the cortex (arrows) and in the spindle (asterisk). (I) Separase appeared on centrosomes (arrow) and chromosomes (asterisk) during mitosis. Scale bar: 10 µm.

To obtain further insight into the sep-1(e2406) mutant phenotype, welocalized the mutant SEP-1 protein by immunofluorescence inembryos incubated at 25°C for 11 hours. In the mutant, SEP-1was still present on the anaphase I spindle (Fig. 8H,I), althoughit was reduced when compared with wild-type embryos. However,we did not detect the mutant protein on cortical granules duringanaphase I (Fig. 8G-I). Therefore, the sep-1(e2406) allele appearsto disrupt separase function partly through disrupting its localizationto cortical granules. The observations that separase localizesto cortical granules and is required for degranulation suggeststhat separase could directly regulate exocytosis.

DISCUSSION

TOP
SUMMARY
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cortical granule exocytosis in C. elegans
Cortical granule exocytosis is a phenomenon observed in theoocytes of many organisms (Wessel et al., 2001). We have identifiedcortical granules in C. elegans and have observed that degranulationoccurs during anaphase I. We observed several steps of corticalgranule trafficking and eggshell formation and identified anumber of OID genes that perturb this process when inactivated (Fig. 9).Several cell cycle genes that cause OID are required for theexocytosis of cortical granules. In particular, separase localizedto cortical granules during anaphase I and was required fordegranulation (Fig. 9). It is possible that OID genes such assecurin, spindle assembly checkpoint components and APC/C affectcortical granule exocytosis partly through regulation of separase.

It will be important to decipher the signals that trigger eggactivation in C. elegans. Oocytes induced to mature by mutantsperm that are incapable of fertilization fail to complete anaphaseI properly, do not form a proper eggshell and do not attemptmeiosis II (McNally and McNally, 2005). Interestingly, corticalgranules were still capable of fusing to the plasma membranein unfertilized oocytes (Sato et al., 2006). As there is nodiscrete cell cycle arrest after maturation in C. elegans (McNally andMcNally, 2005), unfertilized oocytes enter anaphase I. Entry intoanaphase requires separase activation, which triggers degranulation. Furtherstudies are required to understand the nature of the eggshelldefect associated with unfertilized oocytes, and to know whetherCGE is impaired. One possibility is that the wave of exocytosismay not occur with normal kinetics, disrupting eggshell formation.We hypothesize that signals possibly from both ovulation andfertilization stimulate an egg activation pathway acting upstreamof, or in parallel with, separase to coordinate secretion ofeggshell components with cell cycle progression in C. elegans.

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Fig. 8. Separase co-localization during meiosis I in C. elegans. During prometaphase I, the outer kinetochore protein, HIM-10 (A, red), co-localized in cortical filaments with separase (B, green); merge in (C). During anaphase I, cortical granules labeled with WGA (D, red) are also labeled with separase (E, green); merge in F, maximum projection image of four cortical planes. A sep-1(e2406) mutant embryo in anaphase I had cortical granules labeled with WGA (G, red) that were not labeled with separase antibody (H, green), although separase was still present but reduced on the anaphase spindle (arrow); merge in I. Scale bar: 10 µm.

Our data indicate that exocytosis of cortical granules is requiredfor deposition of a mature three-layered eggshell in C. elegans.The outer vitelline layer, which covers oocytes, may functionin sperm binding and restricting the free diffusion of corticalgranule cargo, similar to its role in other species (Wesselet al., 2001

). Interestingly, the vitelline envelope appearsto separate from the plasma membrane at the time of fertilization,which could be part of a mechanism to prevent polyspermy. Ourresults also indicate that degranulation deposits the constituentsof the inner two layers. Complex fibers made up of chitin andprotein arranged in sheets have been observed in other nematodes(Wharton, 1980

). We suspect that the chitin synthase, chs-1, glycosylationenzymes such as sqv-4 and the cpg-1/-2 proteoglycans are involvedin eggshell layer formation (Herman et al., 1999

; Hwang andHorvitz, 2002

; Johnston et al., 2006

; Olson et al., 2006

; Zhanget al., 2005

). As the C. elegans eggshell is permeable untillate meiosis II, an elaborate process is probably involved information of mature eggshell. Further studies will be requiredto define how the secretions from the oocyte are assembled intothe layers of the eggshell.

Secretion during anaphase
Our observations reveal that cortical granule exocytosis occursduring anaphase I and is regulated by separase. There are precedentsfor functions of separase outside cohesin cleavage. For example,in budding yeast, separase plays a non-proteolytic role in theregulation of anaphase spindle dynamics (Higuchi and Uhlmann,2005; Sullivan and Uhlmann, 2003), controls asymmetric spindlepulling forces (Ross and Cohen-Fix, 2004) and activates a signalingpathway that promotes exit from mitosis and cytokinesis (deGramont and Cohen-Fix, 2005; Stegmeier et al., 2002). In frogs,separase plays a role in the centrosome duplication cycle (Tsouand Stearns, 2006). In the mouse, proteolytic-inactive separasecan rescue polar body extrusion but not chromosome segregationin separase-knockout oocytes (Kudo et al., 2006). Separase isrequired for progression through meiosis in both mouse and frog oocytesin part because it binds and inhibits CDK (Gorr et al., 2005; Gorret al., 2006).

We have shown that separase localizes to cortical granules andloss of separase activity reduces exocytosis during anaphaseI. Cortical granule exocytosis during anaphase I might createthe necessary extracellular space, as well as provide additionalmembrane, for polar body extrusion. Consistent with this notion,inactivation of separase dramatically reduced the extracellularspace near the polar body and restricted polar body extrusion (Fig. 6F-K).In sep-1(e2406) mutant embryos the initial separation of homologous chromosomeswas essentially normal, but cortical granule exocytosis wasstill reduced. This is consistent with our observation thatsep-1(e2406) mutant protein does not localize properly to corticalgranules but retains some localization to chromosomes. Theseobservations suggest that the sep-1(e2406) mutation might preferentiallyaffect the role of separase in cortical granule exocytosis whileretaining proteolytic activity toward cohesin. This suggestionis strengthened by the position of the sep-1(e2406) mutation(Siomos et al., 2001), which does not reside in the catalyticdomain, but rather within a large N-terminal domain predictedto contain ARM repeats (Viadiu et al., 2005).

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Fig. 9. Regulation of cortical granule trafficking in C. elegans. Depiction of several steps in cortical granule trafficking and eggshell formation, along with the OID genes involved. Separase localization is indicated. Immature oocytes form cortical granules (red) as they grow while separase remains in the cytoplasm. Just before ovulation, separase accumulates in the nucleus, on oocyte chromosomes (blue) and cytoplasmic filaments. The vitelline layer (brown) separates from the plasma membrane (green) around the time of fertilization (sperm pronucleus in black), and cortical granules cluster near the cortex. Separase is lost from filaments and accumulates on cortical granules as they redistribute in the cortex. Separase is lost during the wave of cortical granule exocytosis in anaphase I. Subsequently, the cargo of cortical granules assembles into the chitin (pink) and lipid (red) layers, which are permeable until late meiosis II.

We observed rare cortical granule exocytic events during anaphaseII in separase mutant and RNAi-depleted embryos (data not shown),further suggesting that cortical granule exocytosis is promotedspecifically during anaphase. The observation that cell cycleregulatory genes control cortical granule exocytosis is surprisinggiven observations made in other organisms. In Xenopus, inhibitingexit from mitosis by a non-degradable cyclin B did not preventcortical granule exocytosis during egg activation (Murray etal., 1989

). Although mouse oocytes can be parthenogeneticallyactivated to undergo degranulation without cell cycle resumption (Ducibellaet al., 2002

), another study indicated that chromosome separationinitiates before cortical granule exocytosis (Tombes et al., 1992

).Studies in hamster oocytes indicated that limited exocytosisof cortical granules over the meiosis I spindle occurs during anaphase,contributing membrane for polar body extrusion (Okada et al.,1986

). These data suggest that cortical granule exocytosis couldalso be regulated by separase during anaphase in oocytes ofother organisms.

The finding that separase regulates cortical granule exocytosisduring anaphase I leads us to speculate that separase may alsoregulate secretion during mitotic cell divisions. This controlmechanism provides an elegant solution for synchronizing membranetrafficking during cell cleavage with chromosome segregationby linking these events through the activity of separase. Wehave observed multinucleate cells in sep-1(e2406) mutants shiftedto the non-permissive temperature after eggshell formation (datanot shown), suggesting that loss of separase activity can cause cytokinesisdefects in mitotic divisions. It is well known that secretionis required during late anaphase and cytokinesis (Albertsonet al., 2005), and separase was identified in a screen for genesrequired for secretion (Bard et al., 2006). Further analysisof how separase promotes exocytosis during anaphase I, and whetherit regulates cytokinesis by a similar mechanism should be afertile focus of future studies.

Supplementary material
Supplementary material for this article is available at http://dev.biologists.org/cgi/content/full/134/21/3837/DC1

ACKNOWLEDGMENTS

We thank Kraig Kumfer for cloning bombardment vectors, HainingZhang for staining protocols and other lab members for feedback;Peter Crump for statistical analysis and Leanne Olds for drawingillustrations; Bill Vogt, Willy Hausner and Mike Szulczewskiof Prairie Technologies (Middleton, WI) for technical assistancewith the swept-field Confocal; Bill Bement, Anna Skop, Bob Goldstein,Ji Liu and Francis Pelegri for sharing equipment, reagents and expertise.The Barbara Meyer lab graciously provided the HIM-10 antibody.cDNA clones were obtained from Yuji Kohara. This work is supportedby the University of Basel to A.S., by the Intramural ResearchProgram at the National Institutes of Health (NIH) NationalInstitute of Diabetes and Digestive and Kidney Diseases to A.G.and C.R., a NIH grant (R01 GM7583) to J.W., a NIH SBIR grant(5R44MH065724) with Prairie Technologies to K.E. and a NIH traininggrant (5F32 GM076867-02) to J.B.

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