C. elegans CLASP/CLS-2 negatively regulates membrane ingression throughout the oocyte cortex and is required for polar body extrusion
Authors:
Aleesa J. Schlientz aff001; Bruce Bowerman aff001
Authors place of work:
Institute of Molecular Biology, University of Oregon, Eugene, OR, United States of America
aff001
Published in the journal:
C. elegans CLASP/CLS-2 negatively regulates membrane ingression throughout the oocyte cortex and is required for polar body extrusion. PLoS Genet 16(10): e32767. doi:10.1371/journal.pgen.1008751
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1008751
Summary
The requirements for oocyte meiotic cytokinesis during polar body extrusion are not well understood. In particular, the relationship between the oocyte meiotic spindle and polar body contractile ring dynamics remains largely unknown. We have used live cell imaging and spindle assembly defective mutants lacking the function of CLASP/CLS-2, kinesin-12/KLP-18, or katanin/MEI-1 to investigate the relationship between meiotic spindle structure and polar body extrusion in C. elegans oocytes. We show that spindle bipolarity and chromosome segregation are not required for polar body contractile ring formation and chromosome extrusion in klp-18 mutants. In contrast, oocytes with similarly severe spindle assembly defects due to loss of CLS-2 or MEI-1 have penetrant and distinct polar body extrusion defects: CLS-2 is required early for contractile ring assembly or stability, while MEI-1 is required later for contractile ring constriction. We also show that CLS-2 both negatively regulates membrane ingression throughout the oocyte cortex during meiosis I, and influences the dynamics of the central spindle-associated proteins Aurora B/AIR-2 and MgcRacGAP/CYK-4. We suggest that proper regulation by CLS-2 of both oocyte cortical stiffness and central spindle protein dynamics may influence contractile ring assembly during polar body extrusion in C. elegans oocytes.
Keywords:
Chromosome structure and function – Caenorhabditis elegans – Meiosis – Cell membranes – Microtubules – Oocytes – Cell polarity – Cellular extrusion
Introduction
Oocyte meiosis comprises a single round of genome replication followed by two highly asymmetric cell divisions that produce one haploid gamete and two small polar bodies that contain discarded chromosomes [1–4]. An acentrosomal spindle segregates homologous chromosomes during the first reductional division, called meiosis I, when half of the recombined homologs are extruded into the first polar body. The equational meiosis II division then segregates sister chromatids, with half extruded into a second polar body and half remaining in the oocyte cytoplasm. Despite being essential for reducing oocyte ploidy, little is known about the cues that organize and influence the actomyosin contractile ring that mediates polar body extrusion.
The dynamics of membrane ingression relative to the oocyte meiotic spindle during polar body extrusion vary from species to species, and the relationships between spindle structure and furrow ingression remain poorly understood [5]. In Caenorhabditis elegans, the oocyte contractile ring initially forms distal to the membrane-proximal meiotic spindle pole, with the spindle axis oriented orthogonally to the overlying cell cortex [5–7]. When observed in utero, the contractile ring ingresses past both the membrane-proximal pole and one set of the segregating chromosomes to then constrict and ultimately separate the nascent polar body from the oocyte [6]. These dynamics contrast substantially with mitotic cytokinesis (Fig 1A), during which signals from astral microtubules and the central spindle position the contractile ring midway between the two spindle poles [8–10]. While the signals required for contractile ring assembly and constriction during mitotic cytokinesis are relatively well understood, how oocyte meiotic spindles influence contractile ring dynamics during polar body extrusion is not known.
Several genes have been shown to be required for polar body extrusion in C. elegans, but how their functions are coordinated remains poorly understood. Similar to mitotic cytokinesis, polar body cytokinesis requires filamentous actin and the non-muscle myosin II heavy-chain NMY-2 and light-chains MLC-4 and MLC-5 [6,11,12]. The cytoskeletal scaffolding protein anillin/ANI-1 facilitates transformation of the initial actomyosin contractile ring into a midbody tube, with anillin depletion resulting in large and unstable polar bodies that often fuse with the oocyte [7]. Consistent with its role as a key activator of cortical actomyosin, the small GTPase RhoA (RHO-1) and its RhoGEF ECT-2 also are required for oocyte polar body extrusion [6,13]. Knockdown of the centralspindlin complex, comprised of MgcRacGAP/CYK-4 and kinesin-6/ZEN-4, results in the assembly of abnormally large contractile rings and a subsequent failure in extrusion [6]. Finally, the chromosomal passenger complex (CPC) member Aurora B/AIR-2 also is required [14].
Formation of the contractile ring distal to both meiotic spindle poles raises the question of how the ring moves relative to the spindle such that it constricts midway between segregating chromosomes. One mechanism proposed for C. elegans is that global contraction of actomyosin throughout the oocyte cortex produces a hydrostatic cytoplasmic force that, combined with depletion of cortical actomyosin overlying the membrane-proximal pole, leads to an out-pocketing of the membrane within the contractile ring that pulls the tethered spindle into the protruding pocket [6,15]. In support of this hypothesis, increased global cortical contractility due to depletion of casein kinase 1 gamma (CSNK-1), a negative regulator of RhoA activity, often results in extrusion of the entire meiotic spindle [15]. However, assessing whether global cortical contractility is required for polar body extrusion has been challenging due to the overlap in requirements for global cortical contractility and polar body contractile ring assembly and constriction.
Despite a stereotyped spatial relationship between the oocyte meiotic spindle and contractile ring assembly and ingression, little is known about how the spindle might influence ring assembly and dynamics. Nevertheless, four observations suggest that in C. elegans, the meiotic spindle provides important cues. First, meiotic spindles that fail to translocate to the oocyte cortex induce the formation of membrane furrows that ingress deeply towards the displaced spindle [6]. Second, loss of the centralspindlin complex, present at the central spindle during anaphase, results in the formation of rings with an abnormally large diameter [6]. Third katanin/mei-1 mutants, which assemble apolar spindles, produce very large polar bodies during meiosis II when microtubule severing is compromised [16]. Finally, while work in mice suggests that chromosomes themselves may provide cues for ring assembly and polar body extrusion via the small GTPase Ran [17,18], knock down of C. elegans RAN-1 does not prevent polar body extrusion [19,20]. These findings suggest that in C. elegans the oocyte meiotic spindle provides cues that influence contractile ring assembly and ingression.
To explore the relationship between meiotic spindle assembly and polar body extrusion, we have examined polar body extrusion in three spindle assembly defective mutants that each lack the function of a conserved protein: CLASP/CLS-2, kinesin-12/KLP-18, or katanin/MEI-1 (Fig 1B). CLASP family proteins promote microtubule stability through their association with microtubules and their tubulin heterodimer-binding TOG (Tumor Over-expressed Gene) domains, decreasing the frequency of microtubule catastrophe and promoting rescue of de-polymerizing microtubules [21–24]. Moreover, human CLASPs have been shown to influence not only microtubule stability and dynamics, but also to interact with actin filaments and potentially crosslink filamentous actin and microtubules [25]. CLS-2 is one of three C. elegans CLASPs and is required for mitotic central spindle stability and for oocyte meiotic spindle assembly and chromosome segregation [26–29]. Vertebrate kinesin-12/KLP-18 family members promote mitotic spindle bipolarity by contributing to forces that push apart anti-parallel microtubules [30–32]. Consistent with such a function, C. elegans oocytes lacking the kinesin-12 family member KLP-18 form monopolar meiotic spindles that draw chromosomes towards a single spindle pole and fail to segregate them [33–35]. The widely conserved microtubule severing complex katanin is encoded by two C. elegans genes, mei-1 and mei-2 [36,37]. Loss of either subunit results in the formation of apolar meiotic spindles that fail to congress or segregate chromosomes [33,38,39], and mutant alleles with reduced microtubule severing extrude abnormally large polar bodies during meiosis II [16].
Here we report our use of fluorescent protein fusions and live cell imaging to characterize polar body extrusion during meiosis I in mutants lacking the function of CLS-2, KLP-18 or MEI-1. Previous studies indicate that both CLS-2 and MEI-1 are involved in polar body extrusion, with oocytes lacking CLS-2 frequently failing to extrude polar bodies [26,29,40], and oocytes lacking MEI-1 forming very large polar bodies [16,41–43]. Furthermore, klp-18 mutants sometimes lack an oocyte pronucleus, suggesting that all oocyte chromosomes can be extruded [33]. However, the process of polar body extrusion has not been directly examined in any of these mutants. Our live imaging of contractile ring assembly and ingression in these three spindle-defective mutant backgrounds shows that bipolar spindle assembly and chromosome segregation are not required for oocyte contractile ring assembly and polar body extrusion. However, CLS-2 is required for contractile ring assembly or stability, and acts as a negative regulator of global cortical membrane ingressions, while MEI-1 may be required late in polar body extrusion for contractile ring constriction. We suggest that CLS-2 influences oocyte cortical stiffness to promote polar body extrusion, and we further suggest that disruption of central spindle-associated protein dynamics may also contribute to proper oocyte meiotic contractile ring assembly and ingression.
Results
CLS-2 is required for oocyte meiotic spindle assembly and polar body extrusion
To investigate the role of CLS-2, we first examined the localization of an extragenic CLS-2::GFP fusion [27] in live oocytes (Fig 2A, S1 Fig, S1 and S2 Movies). Consistent with previous reports, CLS-2::GFP initially localized to meiosis I spindle microtubules and kinetochore cups, and to small patches, previously described as rod-shaped structures or linear elements, dispersed throughout the oocyte cortex [26,44]. Around the time of anaphase onset, the cortical CLS-2::GFP patches disappeared and CLS-2::GFP localized to the central spindle between the segregating chromosomes [29,40]. These results suggest that CLS-2 might have roles not only at the oocyte meiotic spindle but also throughout the oocyte cortex.
Previous studies of CLS-2 requirements, using RNA interference (RNAi) or auxin-induced degradation (AID) of degron tagged CLS-2, have emphasized its central spindle function [26,29,40]. To more definitively assess its roles during oocyte meiotic cell division, we used CRISPR/Cas9 to generate putative null alleles. Each of the four alleles we isolated contains small insertions or deletions that result in frame shifts and premature stop codons before the first TOG domain, likely making them null (Fig 2B, S1 Fig). All are recessive, and homozygous mutant hermaphrodites exhibit fully penetrant embryonic lethality (Fig 2C). To investigate CLS-2 requirements, we have used the cls-2(or1948) allele, and hereafter we refer to oocytes from homozygous cls-2(or1948) hermaphrodites as cls-2 mutants.
We first used ex utero live cell imaging with transgenic strains that express GFP fused to a β-tubulin (GFP::TBB-2) and mCherry fused to a histone H2B (mCherry::H2B) to examine microtubule and chromosome dynamics during meiosis I in control and cls-2 mutant oocytes (Fig 2D; see Materials and methods). Control oocytes formed barrel shaped bipolar spindles that shortened and rotated to become perpendicular to the oocyte cortex prior to anaphase and polar body extrusion (n = 19). Consistent with previous reports [26,29,40], the meiosis I spindles in cls-2 mutants were disorganized and lacked any obvious bipolarity, with chromosomes moving into a small cluster before failing to segregate (n = 13). Furthermore, microtubule levels appeared to be reduced, and quantification of spindle microtubule intensity over time showed a substantial reduction in microtubule levels during meiosis I anaphase compared to control oocytes (Fig 2E). These results are consistent with the established roles of CLASP family members in promoting microtubule stability (see Introduction), and with a previous report that quantified reduced microtubule fluorescence intensity at metaphase in cls-2(RNAi) oocytes [40]. To assess when defects in meiosis I spindle assembly first appear in cls-2 oocytes, we used in utero live cell imaging and observed the early assembly of a normal cage-like microtubule structure that surrounded the oocyte chromosomes, followed by a rapid collapse of this microtubule structure to form an abnormally small cluster associated with the oocyte chromosomes (S1 Fig) (n = 5).
To further examine spindle assembly in cls-2 mutants, we imaged meiosis I in oocytes from transgenic strains expressing an endogenous fusion of GFP to the pole marker ASPM-1 and mCherry::H2B (Fig 2F). As described previously [45], multiple small GFP::ASPM-1 foci coalesced to form a bipolar spindle in control oocytes (n = 14). In cls-2 mutants, the GFP::ASPM-1 foci failed to coalesce to form two spindle poles but rather moved over time to form a single tight cluster of multiple small foci, and chromosomes again moved into a small cluster and failed to segregate (n = 11). We conclude that CLS-2 plays an important role in promoting microtubule stability during meiosis I and is required early for bipolar spindle assembly and chromosome segregation.
In addition to the extensive meiotic spindle defects, we also observed that cls-2 mutants frequently failed to extrude a polar body at the end of meiosis I, consistent with previous reports [26,29]. Control oocytes regularly extruded a polar body at the end of meiosis I, as scored using transgenic strains expressing either GFP::H2B or mCherry::H2B to determine whether oocyte chromosomes remained extruded for the duration of live imaging (93 of 94 control oocytes; Fig 2G; see Materials and methods). In contrast, meiosis I polar body extrusion failed in about 84% of the cls-2 mutant oocytes (80 of 95, Fig 2G).
CLS-2 and MEI-1, but not spindle bipolarity, are required for polar body extrusion
Because the relationship between spindle structure and polar body extrusion is unclear, we next took a comparative approach and also examined meiosis I polar body extrusion after using RNAi to knock down either kinesin-12/KLP-18 or katanin/MEI-1, with knockdown protocols that led to fully penetrant failures in oocyte chromosome segregation (see Materials and methods). As illustrated schematically in Fig 1B, klp-18 mutants assemble monopolar spindles while mei-1 spindles are apolar, and both fail to segregate chromosomes (see Introduction) [33]. We first simply assessed whether polar body extrusion was successful, again using live imaging with transgenic strains expressing either GFP::H2B or mCherry::H2B fusions to score extrusion (Fig 2G). In klp-18 mutants, chromosomes were successfully retained in a meiosis I polar body in 17 of 20 oocytes. In contrast, after MEI-1 knockdown, chromosomes were extruded and retained in a meiosis I polar body in only 5 of 27 oocytes. The absence of meiosis I polar body extrusion in mei-1 mutant oocytes was surprising because mei-1 mutants were originally described as typically having abnormally large polar bodies [41,42], but how often chromosome extrusion into a polar body succeeds or fails has not been reported. Our data indicate that meiosis I polar body extrusion usually fails and suggest that the abnormally large polar bodies observed in mei-1 mutants result from defects in meiosis II, consistent with previous work [16] (see Discussion).
Based on the frequent success of polar body extrusion in klp-18 mutants, we conclude that spindle bipolarity and chromosome segregation are not required for polar body extrusion. Thus, the failed extrusions in cls-2 and mei-1 mutants are not simply due to an absence of spindle bipolarity or a failure to segregate chromosomes.
Meiotic spindle-associated furrows are abnormal in cls-2 and mei-1 mutant oocytes
To better understand the polar body extrusion defects in oocytes lacking CLS-2 or MEI-1, we next examined the spindle-associated membrane furrows that mediate polar body extrusion in transgenic strains expressing mCherry fused to a plasma membrane marker (mCherry::PH) and GFP::H2B (Fig 3A and 3B, S2 Fig, S3 and S4 Movies). In 9 of 16 control oocytes, we observed early membrane furrows that ingressed until they pinched together to encapsulate and extrude chromosomes into the first polar body. In 6 of 16 control oocytes we observed early membrane furrows that were not as clearly resolved in our imaging data but eventually led to polar body extrusion, and in one oocyte furrows were not obvious but a polar body was nevertheless extruded.
In contrast, we observed extensive spindle-associated membrane furrowing defects in cls-2 mutants (Fig 3C–3E, S3 and S4 Figs, S5 and S6 Movies). In 7 of 19 oocytes we observed two furrows in cross-section that retracted before pinching together, one oocyte that formed two furrows that pinched together but failed late in polar body extrusion, and one oocyte that formed two furrows and successfully extruded a polar body (S3 Fig). One of 19 oocytes appeared to form three spindle-associated furrows in cross-section and extruded a polar body (S3 Fig). In 7 of 19 oocytes we observed only a single visible spindle-associated furrow in cross-section that ingressed either to one side of, or directly toward the oocyte chromosomes (Fig 3D, S4 Fig), suggesting that the contractile ring collapsed into a more linear ingressing structure rather than maintaining a ring-like shape. In some cases, when the single ingressing furrow moved directly toward the oocyte chromosomes, it appeared to push chromosomes apart (S4 Fig). Such late separations of chromosomes were observed only in association with ingressing furrows that appeared to be responsible for the chromosome movement. Finally, in one oocyte the membrane dynamics were indistinct, but chromosomes were extruded into a polar body (Fig 3E), and in one oocyte there was no obvious spindle-associated furrowing and polar body extrusion failed (S4 Fig).
In oocytes depleted of klp-18, we observed furrows that more nearly resembled those in control oocytes (Fig 3F and 3G, S5 Fig, S7 and S8 Movies). In 4 of 10 oocytes, we observed two furrows in cross-section that ingressed and then pinched together (Fig 3F), and only 1 of these 4 failed in polar body extrusion. In 6 of 10 oocytes, we observed shallow furrows adjacent to the oocyte chromosomes (Fig 3G), and only 1 of these 6 failed to extrude a polar body.
After MEI-1 knockdown, we observed furrows that initially resembled those in control oocytes but were more widely spaced and often failed late during constriction (Fig 3H–3J, S6 Fig, S9 and S10 Movies). In 2 of 11 oocytes, we observed two furrows in cross-section that ingressed and pinched together to extrude a polar body (Fig 3H). In 3 of 11 oocytes two furrows ingressed and pinched together but then regressed and released chromosomes back into the oocyte cytoplasm (Fig 3I). In 5 of 11 oocytes two furrows ingressed but retracted before pinching together and failed in polar body extrusion (Fig 3J), and finally in 1 of 11 oocytes we observed only a single spindle-associated furrow in cross-section that failed to extrude a polar body.
To summarize, in klp-18 mutant oocytes we observed spindle-associated furrows that usually encapsulated chromosomes and extruded polar bodies, although the oocyte chromosomes were often in close proximity to the membrane with furrows that were shallow and difficult to detect. In cls-2 and mei-1 mutants, meiosis I polar body extrusion frequently failed but we observed distinct defects. While membrane furrowing initially appeared relatively normal but eventually failed in most mei-1 mutant oocytes, cls-2 mutant furrows often appeared abnormal early during ingression and exhibited more severe defects as extrusion attempts progressed.
Polar body contractile ring dynamics are more severely defective in the absence of CLS-2 than in klp-18 or mei-1 mutant oocytes
We next examined assembly and ingression of the contractile ring during oocyte meiosis I, using live cell imaging with transgenic strains expressing both a GFP fusion to the non-muscle myosin II NMY-2 and mCherry::H2B. In 11 of 11 control oocytes, NMY-2::GFP foci initially assembled into discontinuous but discernible rings over the membrane proximal pole, after spindle rotation and before extensive chromosome segregation, and then became more continuous and prominent as they ingressed and constricted between the segregating chromosomes to extrude polar bodies (Fig 4A, S7 Fig, S11 and S12 Movies).
In cls-2 mutant oocytes, the assembly and stability of NMY-2::GFP contractile ring structures were severely defective (Fig 4B, S8 Fig, S13 and S14 Movies). In 7 of 11 oocytes, fragmented or partial contractile rings assembled and 6 of these oocytes failed to extrude a polar body, while 3 of 11 oocytes formed abnormal assemblies of NMY-2::GFP that were more linear and not ring-like, although 2 of these extruded a polar body. Finally, 1 of 11 oocytes formed a relatively normal looking contractile ring that extruded a polar body. The fragmented or partial contractile rings observed in cls-2 mutants often collapsed into single bright foci or bands during constriction.
Contractile ring assembly and dynamics appeared much more normal in klp-18 mutant oocytes (Fig 4C, S9 Fig, S15 and S16 Movies). In 10 of 10 oocytes after KLP-18 knockdown, NMY-2::GFP foci assembled into rings that ingressed and constricted with dynamics similar to those observed in control oocytes, and in 9 of the 10 oocytes chromosomes were stably extruded into polar bodies.
In MEI-1 knockdown oocytes, ring assembly and ingression were much more normal compared to cls-2 mutants, but we nevertheless observed a range of defects and eventual failures to extrude polar bodies (Fig 4D, S10 Fig, S17 and S18 Movies). In 11 of 13 oocytes, the NMY-2::GFP rings that initially formed appeared larger in diameter compared to control oocytes, and in 3 of these 11 oocytes the rings constricted and successfully extruded a polar body. In another 5 of these 11 oocytes, the rings constricted extensively but ultimately regressed and failed at polar body extrusion, while in 3 the rings ingressed and only constricted partially before regressing and failing to extrude polar bodies. Finally, in 2 of 13 oocytes, ring assembly and ingression were more defective and polar body extrusion failed.
To further characterize the polar body extrusion defects in cls-2 mutants, we also examined ring assembly dynamics in transgenic strains expressing mCherry::H2B and mNeonGreen fused to the anillin ANI-1 (mNG::ANI-1), which is dispensable for assembly of the actomyosin contractile ring but required for its conversion from a ring to a tube during constriction [46] (Fig 5A, S19 and S20 Movies). In 10 of 10 control oocytes, mNG::ANI-1 assembled into contractile rings that ingressed and constricted between segregating chromosomes to extrude a polar body, while in 10 of 10 cls-2 oocytes a fragmented contractile ring structure formed and failed to extrude a polar body. We also used two-color live imaging to examine NMY-2::mKate2 and mNG::ANI-1 simultaneously, and observed that these two contractile ring components were co-localized in both control and cls-2 mutant oocytes (Fig 5B, S21 and S22 Movies) (n = 11 control, n = 13 cls-2(or1948)). We conclude that CLS-2 is required for proper ring assembly and ingression dynamics of not only NMY-2 but also ANI-1.
CLS-2 negatively regulates membrane ingression throughout the oocyte cortex during meiosis I
Global contraction of the oocyte actomyosin cortex has been proposed to promote polar body extrusion by generating a hydrostatic cytoplasmic force that produces an out-pocketing of the actomyosin depleted membrane inside the meiotic contractile ring and pulls the membrane-tethered spindle partially into the extruded membrane pocket (see Introduction). To explore the relationship between spindle structure, global cortical contractility and polar body extrusion, we next examined membrane ingressions throughout the oocyte cortex during meiosis I in control and mutant oocytes, using transgenic strains expressing mCherry::PH and GFP::H2B fusions. To document these membrane ingressions, we used temporal overlays of a single central z-plane to portray simultaneously the membrane position at all time points throughout the period of global cortical furrowing. In control oocytes, we observed the spindle-associated furrows and a small number of additional furrows along the oocyte cortex (Fig 6A, S11 Fig) (n = 16).
In contrast, cls-2 mutant oocytes exhibited more extensive cortical furrowing compared to control oocytes (n = 24), while oocytes depleted of either KLP-18 (n = 10) or MEI-1 (n = 14) more nearly resembled control oocytes (Fig 6A, S12 and S13 Figs, S3–S10 Movies). Quantification of global cortical furrowing showed that cls-2 oocytes had significantly more furrows compared to control and klp-18 oocytes (Fig 6B). We conclude that CLS-2 negatively regulates global cortical furrowing, and we suspect that the CLS-2::GFP patches detected throughout the oocyte cortex are responsible for this regulation (Fig 2A, S1 Fig, S1 and S2 Movies; see Discussion).
We next examined the dynamics of the cortical actomyosin cytoskeleton, which mediates the furrowing that occurs throughout the oocyte cortex during polar body extrusion. In control oocytes, NMY-2::GFP (n = 11) and mNG::ANI-1 (n = 10) localized to dynamic patches throughout the oocyte cortex during meiosis I contractile ring assembly and ingression, and then dissipated late in anaphase when global cortical furrowing ends (Fig 6C and 6D, S14 and S15 Figs, S23 and S24 Movies). To determine if the increased global cortical furrowing in cls-2 oocytes is caused by an increase in NMY-2 or ANI-1 patch size or duration, we examined the dynamics of NMY-2::GFP and mNG::ANI-1 and observed dynamics similar to those in control oocytes (Fig 6C and 6D, S16–S18 Figs, S25 and S26 Movies) and did not detect any difference in the area occupied by the cortical NMY-2::GFP or mNG::ANI-1 patches throughout the period of global cortical furrowing and polar body extrusion (S19 Fig). These data suggest that the excess global cortical furrowing observed in cls-2 oocytes is not due to altered NMY-2 or ANI-1 patch dynamics. In contrast, the increased global cortical furrowing observed after knocking down the casein kinase CSNK-1 was associated with altered NMY-2 and ANI-1 cortical patch dynamics and with extrusion of the entire meiosis I spindle into polar bodies [15] (see Discussion).
Loss of CLS-2 results in altered Aurora B/AIR-2 and MgcRacGAP/CYK-4 dynamics
Because (i) cls-2 mutant oocytes fail to assemble a central spindle or segregate chromosomes, (ii) CLS-2::GFP localizes to the central spindle, and (iii) the central spindle-associated proteins Aurora B/AIR-2 and the centralspindlin component MgcRacGAP/CYK-4 are required for polar body extrusion [6,14,26,47], we next considered whether the observed polar body extrusion defects in cls-2 oocytes might be due to altered localization of central spindle proteins to the disorganized spindle microtubules. To address this possibility, we used transgenic strains expressing GFP fusions to either AIR-2 or CYK-4 and examined their localization in control and cls-2 mutant oocytes during the final 360 seconds of meiosis I, when anaphase chromosome segregation, global cortical furrowing, and polar body extrusion occur.
As reported previously [14,26], AIR-2 in control oocytes (n = 12) initially localized to mid-bivalent ring structures before redistributing to the central spindle during anaphase (Fig 7A). In cls-2 mutants (n = 15), despite the lack of spindle organization, GFP::AIR-2 still localized to the mid-bivalent ring structures before redistributing throughout the dis-organized spindle as meiosis I progressed (Fig 7A). Moreover, quantification of the GFP::AIR-2 spindle to cytoplasm fluorescence ratio indicated that cls-2 mutants have increased levels of spindle-associated AIR-2 (Fig 7B).
The centralspindlin complex member CYK-4 localized to the central spindle during anaphase in control oocytes (Fig 7C; n = 12), as reported previously [6,48]. In cls-2 mutant oocytes, GFP::CYK-4 initially localized to the disorganized meiotic spindle, but the levels decreased rapidly over time compared to control oocytes (Fig 7C and 7D).
In summary, the central spindle proteins AIR-2 and CYK-4 show distinct alterations in their localization dynamics in cls-2 mutant oocytes during anaphase of meiosis I. While both are still detected in association with the disorganized mutant spindle, AIR-2 levels were increased and CYK-4 levels decreased relative to control oocytes, raising the possibility that these abnormal dynamics might be at least in part responsible for the contractile ring assembly and polar body extrusion defects in cls-2 mutant oocytes.
Discussion
Remarkably little is known about the relationship between spindle structure and contractile ring assembly and constriction during oocyte meiotic cell division. To gain insight into the cues that influence contractile ring dynamics during polar body extrusion, we have examined ring assembly and constriction in three different C. elegans spindle assembly-defective mutants. Our results indicate that the C. elegans CLASP family member CLS-2 is required not only for assembly of a bipolar meiosis I spindle and chromosome segregation, but also for oocyte meiosis I contractile ring assembly or stability. This requirement for CLS-2 is not due simply to a failure in assembling bipolar spindles or to a lack of chromosome segregation, because monopolar kinesin-12/klp-18 mutant spindles failed to segregate chromosomes but did assemble stable contractile rings that usually extruded chromosomes into a polar body. We have further shown that mei-1/katanin mutant oocytes, which assemble apolar and disorganized oocyte meiosis I spindles, assembled contractile rings that were abnormally large in diameter and usually failed to extrude polar bodies after some ingression, suggesting a later role for MEI-1. In addition, we observed increased cortical furrowing throughout the oocyte cortex during meiosis I in cls-2 mutant oocytes, but not in klp-18 or mei-1 mutants. In mutant oocytes lacking the casein kinase CSNK-1 [15], increased global cortical furrowing is associated with altered cortical actomyosin dynamics and often results in extrusion of the entire meiosis I spindle in C. elegans. However, the increased cortical contractility in cls-2 mutants was not associated with obvious alterations in non-muscle myosin dynamics and was usually associated with complete failures in polar body extrusion. We suggest that, in cls-2 mutant oocytes, altered cortical cytoskeleton dynamics decreases cortical stiffness and thereby disrupts contractile ring assembly and furrow ingression during polar body extrusion. An alternative and not mutually exclusive possibility is that altered relative levels of central spindle proteins disrupts spindle cues that promote ring assembly and ingression.
Using spindle assembly defective mutants to explore contractile ring dynamics during oocyte polar body extrusion
While the requirements for several factors that control oocyte meiotic spindle assembly in C. elegans have been described [1–3], the impact of the resulting spindle assembly defects on polar body extrusion has remained largely unexplored. Indeed, anecdotal observations have suggested that polar body extrusion can occur even in mutants with severe oocyte spindle assembly defects. For example, reducing the function of the microtubule severing complex katanin, comprised of MEI-1 and -2 in C. elegans, results in severely defective apolar spindles that have greatly reduced levels of microtubules and fail to organize or segregate chromosomes and yet often produce abnormally large polar bodies. Similarly, mutant oocytes lacking the kinesin-12 family member KLP-18 assemble monopolar spindles that fail to segregate chromosomes but often produce zygotes that completely lack an egg pronucleus, indicating that all of the oocyte chromosomes are sometimes extruded into polar bodies [33]. In mouse oocytes, DNA-coated beads have been shown to promote the assembly of a polar body-like cortical protrusion, which requires the small GTPase Ran that mediates chromatin signaling and, if allowed to assemble a bead-associated spindle structure, can lead to successful extrusion [17,18]. However, knockdown of the C. elegans Ran family member RAN-1 does not prevent chromosome segregation or polar body extrusion [19,20], suggesting that chromatin cues are not required for contractile ring assembly. Moreover, meiotic spindles that fail to translocate to the oocyte cortex induce the formation of membrane furrows that ingress deeply toward the spindle [6], and C. elegans mutant oocytes lacking central spindle proteins have been shown to produce abnormally large contractile rings that often fail to extrude chromosomes into a polar body [6], suggesting that the oocyte meiotic spindle does influence ring assembly and function.
To explore the relationship between oocyte meiotic spindle structure and membrane ingression during polar body extrusion, we compared polar body extrusion in three C. elegans mutants that are severely defective in oocyte spindle assembly. Because cls-2 mutant oocytes failed to assemble bipolar spindles or segregate chromosomes, we also examined polar body extrusion in klp-18/kinesin-12 mutant oocytes that assemble monopolar spindles and also fail to segregate chromosomes [33–35]. In contrast to cls-2 mutants, in which contractile ring assembly or stability and membrane ingression were severely defective, contractile ring assembly and ingression appeared much more normal in klp-18 mutant oocytes, and chromosomes were usually extruded into a polar body. These findings are consistent with work in cultured mammalian cells showing that cells with monopolar mitotic spindles can still undergo cytokinesis [49]. We conclude that the defects in cls-2 mutant oocytes are not due a failure to assemble a bipolar spindle or to segregate chromosomes, but rather reflect a more specific requirement for CLASP/CLS-2.
A specific requirement for CLS-2 is further supported by our analysis of oocyte meiotic contractile ring assembly and dynamics in katanin/mei-1 oocytes, which assemble spindles that lack any polarity and completely fail to organize the dispersed oocyte chromosomes throughout meiosis I [33,38,39]. Furthermore, similar to cls-2 oocytes, microtubule levels are substantially reduced in mei-1 mutant oocytes [50]. Nevertheless, stable contractile rings usually formed in mei-1 mutant oocytes, although the rings were larger in diameter compared to control oocytes, and we frequently observed extensive furrow ingressions that often enclosed the oocyte chromosomes but usually failed to complete constriction and regressed late in cytokinesis. In the absence of MEI-1, contractile rings can assemble and remain stable until late in meiosis I polar body extrusion, even when oocyte meiotic spindle assembly is at least as severely defective as in cls-2 mutant oocytes.
Contractile ring dynamics during meiosis I were more normal after mei-1 RNAi knockdown compared to cls-2 mutants, but the furrows nevertheless often regressed and polar body extrusion usually failed. Previous studies have shown that partial loss of function mutations in mei-1 result in abnormally large polar bodies that are produced after meiosis II, as a result of decreased microtubule severing that is required for complete disassembly of the meiosis II spindle [16,43]. Our results provide the first systematic examination of polar body extrusion during meiosis I after depletion of katanin/MEI-1, and it is possible that the late failures in polar body cytokinesis that we observed also reflect a requirement for microtubule severing. Alternatively, similar defects were observed in oocytes lacking the centralspindlin components CYK-4 and ZEN-4 [6,14,26,47], and it is possible that central spindle proteins are mis-regulated after MEI-1 knockdown. Further investigation of MEI-1 and its interactions with central spindle proteins should improve our understanding of this late requirement during polar body extrusion.
CLS-2 regulation of oocyte cortical stiffness and contractile ring dynamics
While our analysis indicates that CLS-2 is required early for the assembly or stability of the oocyte meiosis I contractile ring, we do not know if the defects reflect a direct or indirect requirement, or how CLS-2 functions at a molecular level to promote polar body extrusion. Nevertheless, our findings lead us to suggest that CLS-2 may influence polar body extrusion by positively regulating cortical stiffness throughout the oocyte cortex. Based on our observations that (i) the increased furrowing throughout the oocyte cortex is not associated with obvious change in cortical actomyosin dynamics, (ii) CLS-2 localizes to small patches distributed throughout the oocyte cortex, and (iii) CLASP orthologs in other organisms can promote cortical microtubule attachments, we suggest that the increased cortical furrowing in cls-2 mutant oocytes reflects a decrease in cortical stiffness, rather than an increase in cortical actomyosin contractility.
Consistent with our hypothesis that CLS-2 regulates cortical stiffness through regulation of the microtubule and possibly microfilament cytoskeleton, mutations in the Drosophila CLS-2 ortholog Orbit/Mast cause spermatocyte cell division defects associated with a loss of central spindle microtubules that normally promote contractile ring assembly [51,52]. Additionally, human CLASP proteins have been shown to associate with actin filaments and may cross-link microtubules and filamentous actin [25], and mammalian CLASPs have been proposed to link microtubule plus ends with the cell cortex [53,54]. Moreover, oocyte polar body extrusion has been described as a bleb-like process, with local weakening of the actomyosin cytoskeleton inside the contractile ring promoting an out-pocketing of the membrane to form a polar body [5,6]. Studies of bleb formation in other cellular contexts have shown that microtubule destabilization can result in bleb formation [55–57]. Finally, C. elegans CLS-2 has been previously shown to be required for a number of microtubule dependent cortical processes in oocytes, including cytoplasmic streaming and yolk granule packing [58,59]. While it is possible that CLS-2 may act through microtubules to influence cortical stiffness, we have not yet detected significant differences in the levels or organization of cortical microtubules in cls-2 oocytes. Higher spatial and temporal resolution imaging studies might detect subtle changes and prove informative.
Consistent with a role in regulating global oocyte cortical stiffness, we detected CLS-2::GFP in small patches, also referred to as linear elements [44] or rod-shaped structures [26], throughout the cortex in control oocytes. These patches were present early in meiosis I but dissipated before anaphase chromosome segregation, prior to initiation of the membrane ingressions that occur during anaphase in wild-type oocytes. The excessive global cortical furrowing in cls-2 mutants may result from the loss of these cortical patches. Because the patches are undetectable at the time of furrow ingression, we suggest that CLS-2 either acts prior to the initiation of global cortical furrowing or remains present at low and undetected levels to regulate membrane ingression as furrows ingress.
CLS-2 might promote oocyte contractile ring assembly and ingression more directly, through its regulation of microtubule stability during spindle assembly. Astral microtubules associated with this acentrosomal spindle are small and limited in number, but a recent study has proposed that they nevertheless can interact, through dynein, with cortical microtubules to engage pulling forces that move the spindle toward the cortex and rotate it from its initial parallel orientation relative to the oocyte cortex to a perpendicular orientation during polar body extrusion [60]. Astral microtubule interaction with the cortex might then also influence contractile ring assembly. Consistent with such a scenario, we observed CLS-2::GFP throughout the oocyte spindle at the time when contractile ring assembly begins. Higher resolution imaging of the spindle microtubules and their proximity to the cortex in cls-2 mutant oocytes might provide more insight.
Complex regulation of global cortical furrowing during polar body extrusion
Comparing the consequences of reducing the functions of the casein kinase CSNK-1 and of the CLASP family member CLS-2 indicates that the relationship between global cortical dynamics and polar body extrusion is complex. CSNK-1 also limits membrane ingressions throughout the oocyte cortex during meiosis I but appears to do so through negative regulation of actomyosin dynamics, and CSNK-1 knockdown often results in extrusion of the entire meiotic spindle and all of the oocyte chromosomes into the first polar body [15]. These observations support a model in which global cortical contraction generates a hydrostatic cytoplasmic force that promotes an out-pocketing of the plasma membrane that pulls the membrane-tethered spindle pole through the contractile ring and into the forming polar body [6]. While such a mechanism may operate, it also is clear from in utero imaging that the contractile ring and associated plasma membrane ingress substantially prior to constricting roughly midway along the axis of the spindle during polar body extrusion. These dynamics suggest that the spindle and the contractile ring interact to promote furrow ingression and constriction.
The different phenotypes of csnk-1 and cls-2 mutants indicate that negative regulation of global cortical membrane ingression during oocyte meiotic cell division may both promote and prevent the extrusion of chromosomes into polar bodies. These different outcomes presumably reflect differences in how CSNK-1 and CLS-2 influence the cortical cytoskeleton and its dynamics. CSNK-1 appears to regulate cortical actomyosin contractility, while CLS-2 might act through microtubules or microfilaments to promote cortical stiffness, with both influences being important for effective polar body extrusion.
Further investigation of cortical cytoskeleton dynamics, and the interactions of factors that regulate cortical structure and dynamics, should improve our understanding of the relationship between global cortical furrowing and oocyte meiotic contractile ring assembly. Multiple factors, including the kinesin-13 family member KLP-7, the TOG domain protein and XMAP215 ortholog ZYG-9, and Aurora A/AIR-1 have been shown to modulate cortical microtubule levels during oocyte meiotic cell division in C. elegans [20,48,61]. Investigation of how these different cytoskeletal regulators interact may further inform our understanding of polar body extrusion.
Central spindle protein dynamics and polar body extrusion
The abnormal dynamics of the central spindle proteins AIR-2 and CYK-4 in cls-2 mutant oocytes might also contribute to polar body extrusion defects. While extrusion has not been closely examined in oocytes depleted for AIR-2, the extrusion defects in oocytes lacking either CLS-2 or CYK-4 are very distinct. In cyk-4 mutant oocytes, membrane furrows and contractile rings are abnormally large in diameter but otherwise appear normal and ingress before failing to constrict relatively late in extrusion [6]. In cls-2 oocytes, we observed severely abnormal and unstable furrows throughout ingression, with highly defective contractile ring assembly or stability. Thus the cls-2 defects are probably not caused by loss of CYK-4 function, even though CYK-4 levels were substantially reduced during most of anaphase in cls-2 mutants. It seems more likely that either the increased AIR-2 levels, the altered CYK-4 dynamics at the meiotic spindle, or the altered relative levels of AIR-2 and CYK-4, might somehow disrupt contractile ring assembly. Further studies that manipulate AIR-2 or CYK-4 levels, and examine their dynamics in other spindle assembly-defective mutants, may improve our understanding of the relationship between central spindle proteins and oocyte contractile ring assembly.
Materials and methods
C. elegans strain maintenance
All C. elegans strains used in this study (S1 Table), were maintained at 20°C as described previously [62].
cls-2 CRISPR/Cas9 allele generation
Mutations in cls-2 were generated by injecting young adult N2 hermaphrodites with the following mixture [63]: 25μM cls-2 crRNA (ATCAGCCGATCGACTCCGGG), 5μM dpy-10 crRNA (GCTACCATAGGCACCAC GAG), 30μM trRNA, 2.1μg/μl Cas9-NLS, and 2.5μM dpy-10 single-strand DNA (ssDNA, CACTTGAACTTCAATACGGCAAGATGAGAATGACTGGAAACCGTACCGCATGCGGTGCCTATGGTAGCGGAGCTTCACATGGCTTCAGACCAACAGCCTAT). No homologous repair template was used for cls-2, and cls-2 DNA breaks were allowed to repair randomly. Before injection, the trRNA and crRNAs were mixed and incubated at 95°C for 5 minutes, before cooling at room temperature for 5 minutes. After cooling, Cas9-NLS (QB3-Berkeley MacroLab) was added to the annealed trRNA and crRNAs and allowed to incubate for another 5 minutes at room temperature before the dpy-10 ssDNA repair template was added. After injection, hermaphrodites were singled out and their broods were screened for dpy-10 roller or dumpy co-conversion worms, which were allowed to produce broods. Those broods were then evaluated for potential cls-2 phenotypes (embryonic lethality), and lines identified as potentially carrying mutations to cls-2 were balanced. PCR amplified fragments were Sanger sequenced to identify the CRISPR/Cas9-induced mutations.
Feeding RNAi Knockdown of mei-1 and klp-18
RNAi knockdown of mei-1 and klp-18 was achieved by plating hypochlorite synchronized L1 larvae onto E. coli (HT115) lawns induced to express dsRNA corresponding to mei-1 or klp-18 [64]. Plated worms were either maintained at 20°C until adults were imaged (mei-1), or maintained at 20°C and upshifted to 26°C 16 hours prior to imaging (klp-18) to ensure robust knockdown (as determined by the fully penetrant absence of chromosome segregation, indicative of the formation of monopolar meiotic spindles, during both meiosis I and II, after KLP-18 knockdown). The mei-1 RNAi vector was from the Ahringer RNAi library [65]. The klp-18 RNAi vector was made by amplifying a portion of the klp-18 coding sequence from isolated N2 genomic DNA (using primers 5’-ACCGGCAGATCTGATATCATCGATGAATTCTCCAACTTTCAA ATGCCACA-3’ and 5’-ACGGTATCGATAAGCTTGATATCGAATTCCTTCGATATGGAA GAA AGCGG-3’), which was inserted into the L4440 vector backbone using the NEBuilder HiFi DNA assembly cloning kit (NEB).
Live-cell imaging
All imaging was carried out using a Leica DMi8 microscope outfitted with a spinning disk confocal unit–CSU-W1 (Yokogawa) with Borealis (Andor), dual iXon Ultra 897 (Andor) cameras, and a 100x HCX PL APO 1.4–0.70NA oil objective lens (Leica). Metamorph (Molecular Devices) imaging software was used for controlling image acquisition. The 488nm and 561nm channels were imaged simultaneously every 10 seconds with 1μm Z-spacing (either 16μm or 21μm total Z-stacks depending on the fluorescent markers used, with the same stack size used for all movies utilizing the same fluorescent markers).
In utero live imaging of oocytes was accomplished by mounting adult worms with a single row or less of embryos in 1.5μl of M9 mixed with 1.5μl of 0.1μm polystyrene Microspheres (Polysciences Inc.) on a 6% agarose pad with a coverslip gently laid over top. Ex utero imaging of oocytes was carried out by cutting open adult worms with a single row or less of embryos in 4μl of egg buffer (118mM NaCl, 48mM KCl, 2mM CaCl2, 2mM MgCl2, and 0.025 mM of HEPES, filter sterilized before HEPES addition) on a coverslip before mounting onto a 2% agarose pad on a microscope slide.
Image analysis, quantification, and statistical analysis
General image analysis and quantification of microtubules and global cortical furrowing was carried out using FIJI software [66]. Three-dimensional projection and rotation of movies used to look at polar body contractile rings was carried out using Imaris software (Bitplane). Meiosis I polar body extrusion success was evaluated based on whether oocytes extruded any chromosomes marked by GFP or mCherry histone 2B (H2B) into a polar body that remained extruded for the period of imaging, either until meiosis I had obviously ended and meiosis II spindle assembly began, or until pronuclei began to decondense in the one-cell stage embryo after meiosis II. We did not assess polar body extrusion during meiosis II. The end of meiosis I and beginning of meiosis II was considered to be the time at which the chromosomes left in the oocyte cytoplasm began to visibly separate from each other. Projections for spindle-associated furrow examination were made by manually isolating the 5 most spindle-associated z-planes for each time point during the period of global cortical furrowing and then sum projecting the mCherry::PH membrane signal. Membrane temporal overlays were created by overlaying the outlined membrane regions of interest for the period of furrowing (detailed below) to create a single image.
Total spindle microtubule pixel intensity was determined using the following formula: (Mean Grey Value (spindle)/Mean Grey Value (cytoplasm)) × spindle area = total spindle microtubule pixel intensity. The mean grey values for both the meiotic spindle and cytoplasm were determined by drawing a region of interest around either the meiotic spindle or a portion of oocyte cytoplasm devoid of adjacent sperm in maximum projected Z-stacks and measuring the mean grey value of the selected region in ImageJ. Spindle area was determined by measuring the area of the region of interest encompassing the meiotic spindle, or the oocyte chromosomes if the spindle could not be clearly identified (cls-2 mutants).
AIR-2 and CYK-4 fluorescence was quantified similar to above, with the spindle to cytoplasm fluorescence ratio calculated for each time point with the following calculation: (Mean Grey Value (spindle/chromosome associated fluorescence)/Mean Grey Value (bulk cytoplasm)).
The area of cortex covered by NMY-2::GFP or mNG::ANI-1 patches over time was quantified for a subset of movies with low amounts of outside signal from nearby gonad or other embryos, as that signal interferes with image thresholding. Movies were maximum projected in FIJI, and regions of interest were drawn around each timepoint for each oocyte for the 360 seconds prior to the end of meiosis I and beginning of meiosis II (see above). A threshold was applied to each movie using either the Otsu (NMY-2::GFP) or Li (mNG::ANI-1) threshold method with dark background and stack histogram settings. Area of the NMY-2 or ANI-1 thresholded patches was then measured for the drawn regions of interest by limiting the measurements to the threshold pixels and calculating the area fraction.
Quantification of global cortical furrowing was accomplished by drawing regions of interest over the oocyte membrane signal (mCherry::PH) for a single central z-slice for the entire period of global cortical furrowing. Regions of interest were then converted to a high contrast stack of membrane positions over time, which were then analyzed using the ADAPT plugin [67] for ImageJ in order to determine curvature values across the oocyte membrane. A furrow was defined as being at least two consecutive membrane points with negative mean curvature values and a standard deviation of mean curvature at least two standard deviations above the average standard deviation of mean curvature value for the entire oocyte membrane. Membrane points fitting the criteria of a furrow (above) that were separated by a single membrane point not fitting the criteria were considered as part of the same furrow for the purposes of counting. For statistical analysis of global cortical furrowing (Fig 6B), one-way ANOVA was used to determine if there was any difference in the mean furrowing between genotypes, F-Tests to compare the variances, and two-tailed Student’s t-Tests between genotypes to compare the means directly (assuming either equal or unequal variances depending on the F-Test results). All statistical analysis and graphs were completed using Excel (Microsoft).
Supporting information
S1 Fig [a]
CLS-2 localizes to meiotic spindles and is required for their assembly.
S2 Fig [pdf]
Control oocyte spindle-associated membrane furrows.
S3 Fig [pdf]
oocyte spindle-associated membrane furrows.
S4 Fig [pdf]
oocyte spindle-associated membrane furrows.
S5 Fig [rnai]
oocyte spindle-associated membrane furrows.
S6 Fig [rnai]
oocyte spindle-associated membrane furrows.
S7 Fig [pdf]
Control oocyte NMY-2::GFP contractile rings.
S8 Fig [pdf]
oocyte NMY-2::GFP contractile rings.
S9 Fig [rnai]
oocyte NMY-2::GFP contractile rings.
S10 Fig [rnai]
oocyte NMY-2::GFP contractile rings.
S11 Fig [pdf]
Control oocyte membrane temporal overlays.
S12 Fig [pdf]
oocyte membrane temporal overlays.
S13 Fig [rnai]
and membrane temporal overlays.
S14 Fig [pdf]
Control oocyte NMY-2::GFP cortical dynamics.
S15 Fig [pdf]
Control oocyte mNG::ANI-1 cortical dynamics.
S16 Fig [pdf]
oocyte NMY-2::GFP cortical dynamics.
S17 Fig [pdf]
oocyte NMY-2::GFP cortical dynamics.
S18 Fig [pdf]
oocyte mNG::ANI-1 cortical dynamics.
S19 Fig [pdf]
NMY-2 and ANI-1 cortical dynamics.
S1 Movie [green]
CLS-2::GFP localization.
S2 Movie [green]
CLS-2::GFP localization.
S3 Movie [black]
Control oocyte membrane furrowing.
S4 Movie [black]
Control oocyte membrane furrowing.
S5 Movie [black]
oocyte membrane furrowing.
S6 Movie [black]
oocyte membrane furrowing.
S7 Movie [rnai]
oocyte membrane furrowing.
S8 Movie [rnai]
oocyte membrane furrowing.
S9 Movie [rnai]
oocyte membrane furrowing.
S10 Movie [rnai]
oocyte membrane furrowing.
S11 Movie [green]
Control oocyte NMY-2::GFP contractile ring dynamics.
S12 Movie [green]
Control oocyte NMY-2::GFP contractile ring dynamics.
S13 Movie [green]
oocyte NMY-2::GFP contractile ring dynamics.
S14 Movie [green]
oocyte NMY-2::GFP contractile ring dynamics.
S15 Movie [rnai]
oocyte NMY-2::GFP contractile ring dynamics.
S16 Movie [rnai]
oocyte NMY-2::GFP contractile ring dynamics.
S17 Movie [rnai]
oocyte NMY-2::GFP contractile ring dynamics.
S18 Movie [rnai]
oocyte NMY-2::GFP contractile ring dynamics.
S19 Movie [green]
Control oocyte mNG::ANI-1 contractile ring dynamics.
S20 Movie [green]
oocyte mNG::ANI-1 contractile ring dynamics.
S21 Movie [green]
Control oocyte NMY-2::mKate2 and mNG::ANI-1 contractile ring dynamics.
S22 Movie [green]
oocyte NMY-2::mKate2 and mNG::ANI-1 contractile ring dynamics.
S23 Movie [green]
Control oocyte NMY-2::GFP cortical dynamics.
S24 Movie [green]
oocyte NMY-2::GFP cortical dynamics.
S25 Movie [green]
Control oocyte mNG::ANI-1 cortical dynamics.
S26 Movie [green]
oocyte mNG::ANI-1 cortical dynamics.
S1 Table [pdf]
Table of strains used in this study
Zdroje
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