The careful control of Polo kinase by APC/C-Ube2C ensures the intercellular transport of germline centrosomes during Drosophila oogenesis

A feature of metazoan reproduction is the elimination of maternal centrosomes from the oocyte. In animals that form syncytial cysts during oogenesis, including Drosophila and human, all centrosomes within the cyst migrate to the oocyte where they are subsequently degenerated. The importance and the underlying mechanism of this event remain unclear. Here, we show that, during early Drosophila oogenesis, control of the Anaphase Promoting Complex/Cyclosome (APC/C), the ubiquitin ligase complex essential for cell cycle control, ensures proper transport of centrosomes into the oocyte through the regulation of Polo/Plk1 kinase, a critical regulator of the integrity and activity of the centrosome. We show that novel mutations in the APC/C-specific E2, Vihar/Ube2c, that affect its inhibitory regulation on APC/C cause precocious Polo degradation and impedes centrosome transport, through destabilization of centrosomes. The failure of centrosome migration correlates with weakened microtubule polarization in the cyst and allows ectopic microtubule nucleation in nurse cells, leading to the loss of oocyte identity. These results suggest a role for centrosome migration in oocyte fate maintenance through the concentration and confinement of microtubule nucleation activity into the oocyte. Considering the conserved roles of APC/C and Polo throughout the animal kingdom, our findings may be translated into other animals.


Introduction
The centrosome is a major microtubule-organizing centre (MTOC) in many animal cells and, through microtubule nucleation, regulates a wide range of cellular processes during development and in adult tissues [1,2]. The centrosome is composed of a pair of centrioles and an amorphous proteinaceous matrix, the pericentriolar material (PCM), which recruits microtubule-nucleating proteins such as γ-tubulins and also contributes to the stability of centrioles [3,4]. In dividing cells, the centrosomes facilitate the assembly and the orientation of the mitotic spindle, thereby ensuring accurate chromosome segregation and impacting cell fate decision and tissue architecture. In non-dividing cells, centrosomes direct cell migration and intracellular transport by forming the polarized microtubule network, or alternatively centrioles are converted to basal bodies to form primary cilia. Centrosome dysfunction is linked to various human diseases including cancer, microcephaly and ciliopathy [1,5].
In the fruit fly Drosophila melanogaster, the centrosome has been implicated in the development of the oocyte through their microtubule-organizing capabilities [6,7]. The Drosophila oocyte develops through 14 stages that are delineated by morphological changes of egg chambers [8,9]. In each ovariole, oogenesis starts at the anterior tip in the germarium where the female germline stem cell resides and divides asymmetrically to produce a daughter stem cell and a cystoblast. The cystoblast then undergoes exactly four rounds of mitotic divisions with incomplete cytokinesis to create a 16cell syncytial cyst, in which only one cell eventually becomes the oocyte, whereas the other 15 cells take on a nurse cell fate. During this process, germline centrosomes of the 16 cystocytes exhibit a very peculiar behaviour: virtually, all the 32 centrosomes intercellularly migrate within the cyst to eventually accumulate in one cell, the future oocyte [7]. This migration coincides with the events that mark the specification of the oocyte: the concentration of fate determinants such as Bicaudal-D (BicD), Egalitarian (Egl) and Oo18 RNA-binding protein (Orb) [10][11][12][13], and the restriction of synaptonemal complexes to the oocyte [14]. These observations suggest potential involvement of germline centrosomes in the specification and/ or the subsequent differentiation of the oocyte [6]. Importantly, the centrosome migration following the syncytial cyst formation is likely to be a universal feature of oogenesis as it is observed in animals as diverse as fish and mammals [15,16]. However, despite the universality of this phenomenon, its significance, as well as the molecular mechanism directing this process, remains elusive.
The microtubule cytoskeleton plays a critical role in Drosophila oogenesis [17,18]. Shortly after the formation of the 16-cell cyst, microtubules start nucleating in the presumptive oocyte and subsequently form an oocyte-centric polarized network that runs through the cyst, which is believed to be required for oocyte maturation as well as the subsequent establishment of the body axes of the embryo [9,19,20]. Given the established role of the centrosome as a major MTOC, it has been postulated that centrosomes may be involved in the formation and/or the maintenance of this oocyte-centred microtubule network through their microtubule nucleation activity [6,17,21]. Nevertheless, the study using loss-of-function mutations in sas4, a gene required for centriole duplication, demonstrated that the oocyte develops normally in homozygous sas4 mutant flies, despite virtually no detectable centrioles in the female germlines [22]. Moreover, it is widely acknowledged that germline centrosomes are degenerated by the end of oogenesis and do not contribute to the embryo. It was recently demonstrated in Drosophila that forced retention of centrosomes in the oocyte results in meiotic defects and subsequent sterility [23]. Thus, there is a clear paradox: if the centrosomes are unnecessary for oocyte development, and even detrimental to embryogenesis, why do they need to be transported into the oocyte? Why is such a seemingly wasteful phenomenon conserved through evolution?
In our previous study, we showed that the centrosome migration requires neither microtubule polymerization nor the activity of BicD and Egl, but does the function of the minus end-directed microtubule motor dynein [24]. It was also reported that mutations in the large cytoskeletal linker, spectroplakin family protein, Short stop (Shot), block the centrosome migration [25]. However, the function of dyneins is also required for the normal morphology of the fusome, the germline-specific membranous organelle that forms a large branched network throughout the cyst and plays a critical role in the asymmetric division of cystoblasts as well as in the specification of the oocyte [21,24,26]. In the shot mutants, although the fusome structure appears unaffected, the polarized microtubule network is not formed and the fate markers do not accumulate in the oocyte [25]. Thus, the interdependency between the events that coincide upon oocyte specification has been a stumbling block for assigning a specific role for the centrosome migration during Drosophila oogenesis.
Both the biogenesis and the microtubule nucleation activity of the centrosome are tightly coupled to the progression of the cell cycle. An E3 ubiquitin ligase complex, Anaphase Promoting Complex/Cyclosome (APC/C), plays a central role in this coupling. Besides many proteins involved in cell cycle regulation, the APC/C also targets proteins that are critical for centriole biogenesis, such as Sas6, STIL and Securin, and for microtubule nucleation, such as Plk1, Aurora A and Spd2, for proteasome-mediated destruction within specific time windows during the cell cycle [27][28][29][30][31][32]. Conversely, APC/C activity is also regulated by the centrosome: the local activity of APC/C at centrosomes depends on the physical interaction between an APC/C regulatory subunit and a centrosome component [31,33]. Ube2C is the E2 ubiquitinconjugating enzyme that is specifically required for the E3 ubiquitin ligase activity of APC/C [34,35]. The cellular levels of Ube2C oscillate during the cell cycle through its autoubiquitination, peaking at mitosis and dropping in the G1 phase [34,36,37]. Importantly, in Drosophila and mammalian cells, Ube2C is enriched at the centrosome and its over-expression leads to the amplification of centrosomes [34,38]. Moreover, excess Ube2C increases sporadic tumour formation in mice and over-expression of Ube2C is associated with various human cancers [38,39]. Therefore, strict control of Ube2C activity is critical for the tight coupling of the centrosome cycle to the cell cycle as well as for tumour suppression. However, the target(s) of the APC/C Ube2C that is critical for centrosome integrity is as yet unidentified.
In this study, we report novel mutants of Drosophila Ube2C Vihar (Vih), vih ΔN , generated by CRISPR genome editing, in which the centrosome migration is intervened in the female germline, despite apparent intact fusome structure and proper oocyte specification. We show that vih ΔN mutations probably cause the upregulation of APC/C, which in turn leads to the reduction of Polo kinase, one of the APC/C substrates and the critical regulator of the integrity and microtubule nucleation activity of the centrosome, in developing egg chambers. The reduction of Polo interferes with the transport of centrosomes into the oocyte, probably through destabilization of germline centrioles. We further show that, in the vih ΔN mutant egg chambers with mislocalized centrosomes, the polarized microtubule network is weakened and microtubule nucleation occurs at ectopic centrosomes in nurse cells, resulting in the loss of oocyte fate and the disruption of the oocyte-nurse cell membranes. These results point to the critical importance of the centrosome transport for the spatial regulation of microtubule nucleation during the early oocyte development in Drosophila, which is orchestrated by the evolutionarily conserved pathway: APC/C Vih -Polo pathway.

N-terminal deletion mutations in Drosophila vih gene cause defects in early oogenesis
To investigate the function of the APC/C-dependent regulation of centrosomes in animal development, we generated novel mutations in the APC/C-specific E2 enzyme, Vih, using the CRISPR genome editing technique in Drosophila [40]. We targeted the conserved 27-amino acid N-terminus extension of the Vih protein, which is unique to the Ube2C family E2s and is involved in auto-inhibition of the APC/C [37,41] (figure 1a). We have generated a series of vih alleles, of which two are null alleles (vih Null ), caused by frame-shifts, and the other two are in-frame deletions which lack four or nine residues in the N-terminal extension (vih ΔN-4 and vih ΔN-9 ; figure 1b; see Material and methods for detailed characterization). vih Null homozygous mutants were lethal at the pupal stage and showed various mitotic phenotypes, such as overly condensed chromosomes, lagging chromosomes and supernumerary centrosomes, in the larval neuroblasts, similar to the previously reported vih null alleles (electronic supplementary material, figure S1) [34]. By contrast, both vih ΔN mutants are homozygous viable and develop into adulthood. The endogenous expression of the truncated forms of Vih proteins was confirmed by western blot using the lysates of the vih ΔN mutant ovaries (figure 1c). vih ΔN adult flies appear morphologically normal, except for occasional minor defects. However, the females of both vih ΔN mutants showed a substantial decrease in cumulative fecundity (total number of eggs laid), down to 55% of control (figure 1d). Homozygous and heterozygous vih ΔN-9 mutants showed comparable levels of fecundity reduction (figure 1d), suggesting a potential dominant effect of the mutation. In addition, while the majority of eggs laid by vih ΔN females could produce larva, a small proportion of eggs showed dorsal appendage defects (9%, n = 836, data not shown), indicative of dorsal-ventral polarity abnormalities, which are frequently caused by a defect in the microtubule-dependent patterning of the egg chamber [18]. These data suggest defects in oogenesis in vih ΔN mutant females.
To elucidate the cause of the reduced fertility, we examined developing ovaries in vih ΔN homozygous mutants. The Drosophila oocyte undergoes 14 developmental stages (S1-14; figure 2a) [8,9]. We found that a large proportion of vih ΔN egg chambers exhibit severe structural abnormalities as early as in S3 (figure 2b,c). While follicular epithelia, with a somatic origin, maintain the intact monolayer, the germline cell membranes that intervene the oocyte and nurse cells ('oocyte-nurse cell membranes', hereinafter) start collapsing after S3 and subsequently form large aggregates in the centre of the egg chambers (figure 2b, white arrows; electronic supplementary material, movies S1 and S2). This phenotype was observed in egg chambers in both homozygous and heterozygous, vih ΔN-9 and vih ΔN-4 mutants (figure 2b) and increased with age (electronic supplementary material, figure S2). As this phenotype resembles that of mutations that affect   The quantification of ovarioles that exhibited the membrane phenotype. The proportion of ovarioles with the membrane phenotype was determined for each of the genotypes indicated. (d ) Germarium-S1 and S4 control and vih ΔN-9 egg chambers stained for DNA (DAPI) in blue, fusome (Hts) in green, and F-actin (Phalloidin) in red, and centrioles (Asl) in white (arrowheads indicate centrioles and asterisks the oocyte). (e) The quantification of centrosome puncta (stained with Asl) in S1-3 control and vih ΔN-9 egg chambers, significance determined using Welch's t-test for the control compared with the phenotype ( p = 5.0 × 10 −6 ) and with Wilcoxon signed-rank test with the control to no phenotype ( p > 2 × 10 −1 ). All scale bars equal to 10 µm.
royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 membrane integrity (for example, rab6 D23D mutations) [42], hereinafter, we refer to this phenotype as the 'membrane phenotype'. Considering its high frequency and severity, we conclude that the membrane phenotype is the main cause of the reduced fertility rate in vih ΔN mutant females. Because of the higher penetrance of the phenotype in vih ΔN-9 mutants than in vih ΔN-4 mutants, we focus our subsequent analysis on vih ΔN-9 mutants unless stated otherwise.

Centrosome transport is compromised in vih ΔN egg chambers
To determine the primary cause of the membrane phenotype, we examined the vih ΔN mutant germline earlier than S3 when the disruption of the oocyte-nurse cell membranes becomes apparent. At the start of oogenesis, germline stem cells located at the anterior tip of the germarium divide asymmetrically to generate cystoblasts, which in turn undergo exactly four rounds of mitotic division without complete cytokinesis to form 16 syncytial cytocytes ( figure 2a). In all the vih ΔN-4 and vih ΔN-9 germline cysts examined, 16 cells were detectable, as in control (figure 2b), confirming our result that vih ΔN mutations do not block mitotic division (electronic supplementary material, figure S1). We next examined the centrosomes within the cyst in vih ΔN mutants. After the cyst formation, centrosomes within the 16 cells of the cyst migrate intercellularly through ring canals and accumulate in one cell, the presumptive oocyte (figure 2a) [7]. We visualized centrosomes by immunostaining against the centriole component Asterless (Asl) [43], and found that, in control S1-3 egg chambers, the majority of centrosomes were located in the presumptive oocyte, in which they subsequently clustered at the posterior region (figure 2d,e; electronic supplementary material, movie S3). However, in a large proportion of vih ΔN-9 S1-3 egg chambers, the majority of centrosomes were retained by nurse cells, often adjacent to ring canals (figure 2d,e). Even the centrosomes that had reached the oocyte were frequently mispositioned, lingering around in the anterior region (figure 2d; electronic supplementary material, movie S4). Thus, germline centrosomes fail to migrate properly from nurse cells to the oocyte in vih ΔN mutant egg chambers. Importantly, the incidence of this centrosome migration defect in early-stage egg chambers tightly correlates with the appearance of the membrane phenotype in later stages in the same ovarioles: in the vih ΔN-9 ovarioles that exhibited the membrane phenotype after S3, average 9.2 centrosome clusters were present in the S1-3 egg chambers while the ovarioles with no membrane phenotype showed average 3.5 centrosome puncta, comparable to the control (figure 2e). This coexistence of the two phenotypes within the same ovarioles suggests a potential causal link between the centrosome transport defect in early egg chambers and the membrane phenotype in later-stage egg chambers in vih ΔN mutants.

Destabilization of centrosomes interferes with their migration in vih ΔN egg chambers
The mechanism underlying the centrosome transport is largely unknown. Thus, to gain insight into the molecular mechanism, we wished to determine how vih ΔN mutations impede the centrosome transport. We previously showed that the centrosomes cannot migrate into the oocyte in germline clones with a mutation in Dynein heavy chain 64C (Dhc64c), suggesting that the function of the minus end-directed microtubule motor dynein is required for the centrosome migration [24]. However, in the Dhc64c mutant germarium, the fusome becomes prematurely fragmented during the time when centrosomes migrate [24]. It was observed that centrosomes migrate along the fusome [17,21]. Thus, to test if the centrosome migration defect in the vih ΔN mutant may be caused by the disruption of the fusome, we examined the fusome structure. Unlike the Dhc64C mutations, the morphology of the fusome appears normal in vih ΔN-9 germaria: its branching network that extended throughout the cyst was clearly observed in Region 2 (electronic supplementary material, figure S3A,B), and centrosomes were found attached to the fusome, similar to control (n = 17; electronic supplementary material, figure S3A). Thus, it is unlikely that the centrosome migration defect observed in the vih ΔN mutant germlines is caused by the disruption of the fusome. We next turned our attention to the germline centrosomes themselves. We noted that the intensity of Asl signals is generally lower in vih ΔN egg chambers than in control. In addition, we found that Asl signals, hence centrosomes, disappear earlier in vih ΔN egg chambers than in control: in control egg chambers, a cluster of centrosomes were detectable in the oocyte until S12 before being gradually degenerated, as reported previously [23], whereas, in vih ΔN-9 egg chambers with the membrane phenotype, centrosome signals were reduced after S6 and virtually undetectable after S9 (figure 3a). However, the expression levels of Asl proteins in the lysates from vih ΔN and control ovaries were comparable (figure 3b). These data suggest that centrosomes may be structurally unstable in vih ΔN egg chambers.
We speculate that this destabilization of germline centrosomes observed may underlie the centrosome migration defect in vih ΔN egg chambers. We reasoned that, if the instability of centrosomes is indeed a cause of the centrosome migration defect, further destabilizing the centrosomes may enhance the occurrence of the centrosome migration failure in the vih ΔN-9 mutants. To test this, we decided to reduce the dosage of Sas4 protein, a core centriole component that is also required for the PCM recruitment during mitosis [44,45], to destabilize germline centrioles. We found that removing one functional copy of sas4 gene by using a loss-of-function allele (sas4 s2214 ) significantly increased the proportion of ovarioles exhibiting the membrane phenotype (45-73%, p = 0.0002; figure 3c,d), concurrently with centrosome migration defects (figure 3e). Meanwhile, in the wild-type background, the heterozygous sas4 s2214 mutation caused neither of these phenotypes (figure 3c-e). This result supports our hypothesis that centrosome instability may underlie the failure in the centrosome transport in the vih ΔN mutant germline. Furthermore, the persisting coexistence of the centrosome migration defect and the membrane phenotype observed in sas4 s2214 /+; vih ΔN-9 ovaries further supports the possible causality between these two phenotypes.

A reduction of Polo kinase impedes the germline centrosome transport
An evolutionarily conserved kinase Polo (Plk1 in human) is a key regulator of centrosomes which recruits the PCM to the centrioles by directly phosphorylating Sas4 [46]. A recent royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 study identified Polo as a key regulator of the stability of centrosomes in the Drosophila female germline: it was shown that downregulation of Polo by RNA interference causes premature shedding of the PCM, leading to an early elimination of centriole from the oocyte, while tethering Polo to centrioles stabilizes the centrosomes, allowing their persistence beyond oogenesis, even in the mature egg [23]. Therefore, we suspected that Polo function may be altered in vih ΔN egg chambers, which causes destabilization of centrosomes.
We examined the expression levels of endogenous Polo proteins in vih ΔN mutant ovaries to find a significant reduction of Polo levels in vih ΔN-9 ovary extracts, compared to control (figure 4a; electronic supplementary material, figure S4). Next, to determine if the reduced Polo levels can account for the vih ΔN-9 phenotypes, we tested whether increasing the expression levels of Polo, by introducing a functional polo transgene (GFP-polo) [46], could rescue the centrosome migration defect and the membrane phenotype. We found that two vih  (n = 55) The quantification of centrosome puncta in S1-3 egg chambers, significance determined using a Wilcoxon signed-rank test ( p < 0.001). All scale bars equal to 10 µm.
royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 copies of GFP-polo in the vih ΔN-9 background were able to completely rescue the membrane phenotype (0%, n = 60; figure 4b, c) and bring the centrosome transport efficiency back to the control level (average 3.1 puncta, n = 21; figure 4b,d). These data suggest that the reduction of Polo may be the main cause of the centrosome transport defect in the vih ΔN egg chambers, probably through destabilization of germline centrosomes. It is noteworthy that the wild-type flies carrying GFP-polo transgene showed less centrosome puncta (1.1 puncta, n = 21; figure 4d) than those without the transgene (3.2 puncta, n = 61; figure 4d) in early egg chambers, suggesting that higher expression of Polo may accelerate the centrosome migration into the oocyte.    This result also suggests that Polo may regulate the centrosome transport during normal oocyte development. To directly test this notion, we investigated the centrosome transport in egg chambers in polo hypomorph mutants. The transheterozygous mutants carrying hypomorphic ( polo 1 ) and amorphic ( polo 11 ) alleles are viable but are sterile [47]. polo 1 /polo 11 mutant egg chambers exhibited highly pleotropic phenotypes, including mitotic defects of cystoblasts (figure 4e). Thus, to specifically address the Polo function in the centrosome migration and later oocyte development, we focused our subsequent analysis on egg chambers containing 16 cells, which indicate the successful completion of four rounds of mitotic division (43%, n = 104). In this population, we observed an average of 9.5 centrosome puncta within S1-3 egg chambers (n = 21; figure 4d,e), indicating a defect in centrosome migration similar to vih ΔN mutants. Furthermore, we also found that membranes between nurse cell were disrupted in a large fraction of mid-to-late stage egg chambers (66.7%, n = 26), although less severe compared to vih ΔN mutants (figure 4f,g). All together, these results strongly suggest that Polo is the key regulator of centrosome migration within the germline cyst, whose protein levels are reduced in the vih ΔN mutant female germline. Proper transport of centrosomes to the oocyte or normal levels of Polo may be critical to maintain the integrity of nurse cell membranes during the later stage of oocyte development.

Vih Δn mutations cause the upregulation of APC/C, leading to premature Polo degradation
We next asked how vih ΔN mutations cause the Polo reduction. As Polo orthologues are known to be targets of the APC/ C-dependent degradation in other species including human cells [48,49], we speculated that Polo might be prematurely degraded by APC/C in vih ΔN mutants. It was previously shown that the N-terminal extension conserved among the Ube2C family of E2 enzymes is not essential for the E2 catalytic activity of human Ube2C (also known as UbcH10) but rather important for negatively regulation of the APC/C by human Ube2C [37,41]. We therefore hypothesized that the vih ΔN mutations may specifically abolish the APC/C-inhibitory function of Vih, thereby causing APC/C upregulation in vivo. We confirmed that Vih ΔN is indeed as catalytically active as Vih WT in a reconstituted APC/C-dependent ubiquitination assay using Drosophila APC/C that was purified from Drosophila embryos (see Methods for the detailed protocol; figure 5a,b): the ubiquitination activity of APC/C-Vih ΔN-9 (lanes 13-16, figure 5a) on a model APC/C substrate, Mes1, was comparable to APC/C-Vih WT (lanes 9-12) while catalytically inactive Vih ΔCS (lanes 17-20) did not support ubiquitination of Mes1. Next, we monitored APC/C activity in vivo by analysing the endogenous levels of CycB, a known APC/C substrate, in ovaries. We observed an apparent reduction in CycB levels in vih ΔN ovary extracts compared to control, in support of the upregulation of APC/C activity in vih ΔN ovaries (figure 5c). Finally, to test if the vih ΔN phenotypes are caused by deregulated APC/C activity, we reduced APC/C activity by halving the dose of the gene encoding the APC/C catalytic subunit, morula (mr), in the vih ΔN-9 homozygous background. We found that the heterozygous mr mutation strongly suppressed both the membrane phenotype and the centrosome migration defect (figure 5d-f). Similar suppression of the vih ΔN-9 phenotypes was also observed by over-expression of the canonical APC/C substrate Cyclin B, which inhibits the degradation of other APC/C substrates through competition for the binding sites on the APC/C (data not shown). Collectively, these data strongly suggest that vih ΔN mutations cause the upregulation of APC/C in the germline cyst, probably through the loss of negative regulation of the APC/C by Vih. This deregulation of APC/C leads to the destabilization of its substrate Polo, which in turn impedes the centrosome transport.
2.6. The centrosome migration may be important for the maintenance of oocyte fate As shown above, vih ΔN mutations prevent the centrosome transport without affecting the fusome structure, unlike previously reported Dhc64c mutations [50] (figure 2d,e; electronic supplementary material, figure S3). Thus, further characterization of vih ΔN mutant phenotypes may provide a novel insight into the specific role of the centrosome migration in the Drosophila oocyte development. We examined midto-late stages (S3 onwards) of vih ΔN egg chambers and noted that many vih ΔN egg chambers have no distinguishable 'oocytes' (based on the size and the morphology of the nucleus). We therefore tested if an oocyte is properly selected among the 16 cells of the cyst in vih ΔN egg chambers by staining Orb, an oocyte fate marker that is localized in the oocyte cytoplasm [12]. In all the vih ΔN-9 S1 egg chambers examined, including those in the ovarioles displaying the membrane phenotype, Orb accumulated strongly in the cytoplasm of a single cell in each cyst, indicating that the oocyte is properly specified within a cyst in vih ΔN egg chambers (figure 6a). However, in The quantification of ovarioles that exhibited the membrane phenotype in indicated genotypes (n indicates total sample number in two biological replicates). Significance determined using a Student t-test ( p < 0.001). (d ) The quantification of ectopic centrosome puncta stained with Asl in S1-3 control, vih ΔN-9 , GFP-polo and GFP-polo;; vih ΔN-9 , polo 1 / TM6B, and hypomorph polo mutant ( polo 1 / polo 11 ) egg chambers. Significance determined using a Wilcoxon signed-rank test ( p < 0.005). (e) polo 1 /TM6B and polo 1 /polo 11 egg chambers stained for DNA (DAPI) in blue, F-actin (Phalloidin) in red and centrioles (Asl) in white (arrowheads indicate centrioles and asterisks oocytes). Scale bars equal to 10 µm. ( f ) The quantification of the membrane disruption phenotype. The percentages of control (w 1118 , n = 38) and polo 1 /polo 11 (n = 39) ovarioles containing mid-late stage (after S4) egg chambers exhibiting disruption of nurse cell membranes were quantified. # p-value ≤ 0.0001. (g) Examples of nurse cell membrane disruption observed in mid-late stage (after S4) polo 1 /polo 11 egg chambers stained for DNA (DAPI) in blue, F-actin (Phalloidin) in red. White arrowheads indicate nurse cells with disrupted membranes.
royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 95% of vih ΔN-9 ovarioles exhibiting the membrane phenotype (n = 38), Orb failed to remain localized in the oocyte after S3 and spread weakly through the entire cytoplasm, frequently forming ectopic foci around centrosome/F-actin aggregates in the middle of the egg chamber ( figure 6a,b). We also checked whether oocytes keep arrested in meiotic prophase I in vih ΔN-9 egg chambers, by analysing the expression of the cell cycle markers, Dacapo (Dap) and Cyclin E (CycE) [51]. In all control egg chambers examined, both cell cycle markers localized to the germinal vesicle in the oocyte from early to late oogenesis (n = 100; figure 6c,d). By contrast, in 86% of vih ΔN-9 egg chambers (n = 56), there was no obvious Dap and CycE accumulation within the germinal vesicle after S3 and the oocyte appeared to become polyploid through endocycle as nurse cells ( judged by its nuclear size) ( figure 6c,d). Thus, the oocyte is initially specified but subsequently lose its identity in the vih ΔN-9 germline. Since we also observed the centrosome migration defect in polo mutant ovaries ( polo 1 /polo 11 , figure 4d,e), we also examined the maintenance of oocyte identity in polo mutant egg chambers by analysing Orb localization. We found that a small but statistically significant fraction of egg chambers (after S4) had no oocytes (cells with Orb accumulation) or more than one oocytes in the polo ovaries (18%, n = 39, p = 0.0146; figure 6f,g). Together, these results suggest that the migration of centrosomes into the oocyte may be critical for the maintenance of oocyte identify after it is specified within the cyst in the germarium.
As shown above, nurse cell membranes are often disrupted in vih ΔN and polo mutant egg chambers (figures 2b,c and 4f,g), it may be possible that the loss of oocyte fate in these mutant egg chambers is caused merely by the disruption of the oocyte-nurse cell membranes (i.e. the membrane phenotype), allowing the dispersal of oocyte determinant factors from the oocyte cytoplasm. To test whether membrane breaking is indeed accountable for the oocyte loss, we examined egg chambers carrying a mutation in a small GTPase Rab6 (rab6 D23D ), which causes the membrane disruption in the germline cyst, due to defective membrane trafficking [42]. We generated homozygous rab6 D23D mutant germline clones using the FLP/FRT system [52]. As reported previously, oocyte-nurse cell membranes as well as membranes between nurse cells started collapsing in the mutant egg chambers after S3, similar to vih ΔN egg chambers (figure 6e).  royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 Nevertheless, in the majority of the rab6 D23D mutant egg chambers including those in which the oocyte-nurse cell membranes were partially raptured, oocytes were still clearly identifiable by their compact nuclear size and Orb accumulation around the nuclei until late stages (93%, n = 56, figure 6b,e). This is in stark contrast to vih ΔN-9 and polo 1 / polo 11 mutants where Orb localization is almost entirely lost in egg chambers ( figure 6a,b,f,g). Thus, although we cannot completely rule out the possibility, membrane breaking is unlikely to be accountable, at least solely, for the oocyte fate loss in vih ΔN and polo mutant egg chambers.
2.7. The centrosome transport may promote the formation of the polarized microtubule network in the germline cyst The tight correlation between centrosome migration defects, membrane disruption and oocyte fate loss observed in vih ΔN and polo mutant germlines suggests a possible causal relationship between these phenotypes. It is known that, shortly after the oocyte is specified within a cyst, microtubules start to accumulate in the oocyte and form a polarized network that emanates from the oocyte and extend through the whole cyst. This oocyte-centric polarized network is believed to be required for oocyte maturation by mediating the directed transport of various proteins and RNAs, including oocyte fate markers, in developing egg chambers [9,19,20]. It has been postulated that, while the microtubule nucleation activity of germline centrosomes appears to be inactivated during migration, it may be reactivated in the oocyte and promote the formation of the polarized microtubule network [6,17,21]. We therefore hypothesized that the failure in centrosome migration into the oocyte may interfere with the establishment of the oocyte-centric polarized microtubule network within the egg chamber. This can explain the correlation between the centrosome migration defect and the loss of oocyte identity in vih ΔN and polo mutant ovaries.
To test this hypothesis, we first monitored microtubule structures in fixed preparations of vih ΔN egg chambers. In control S4-6 egg chambers, microtubules were highly accumulated in the oocyte and some pools of the microtubules appeared to be nucleated in the vicinity of centrosome clusters, which were located in the posterior region of the oocyte (figure 7a, control). By contrast, in all S4-6 vih ΔN-9 egg chambers exhibiting the membrane phenotype, no specific accumulation of microtubules was observed within egg chambers and only short microtubule bundles grew from some of ectopic centrosomes (figure 7a, vih ΔN-9 , Stage 4-). However, in all early S1 egg chambers before membranes start collapsing, the accumulation of microtubules in the oocyte was visible in both control and vih ΔN mutants (figure 7a, Stages 1-3), suggesting that microtubules start nucleating in the oocyte and start forming a network in vih ΔN egg chambers. Thus, we next assessed whether the microtubule network is properly polarized within the cyst by examining the localization of the minus end-directed microtubule motor dynein (Dhc64C) [53]. As reported previously [53], in control egg chambers, Dhc64C signals were accumulated at the periphery of the germinal vesicle during S1-3 and continued being enriched in the oocyte cytoplasm until late stages ( figure 7b,c), indicative of the polarization of microtubules with their minus end oriented to the oocyte. However, in vih ΔN-9 S1-3 egg chambers (with still detectable oocyte-nurse cell membranes), we found a significant reduction in the Dhc64C localization in the oocyte (figure 7b,c), indicating reduced microtubule polarization. Thus, in the vih ΔN egg chambers, although the microtubule network begins to form, it is not properly (at least not fully) polarized. Since the polarized microtubule network is crucial for the directed intercellular trafficking of various materials, including oocyte determinants, between the oocyte and nurse cells [9,19,20], this reduced microtubule polarization is likely to account for the subsequent loss of oocyte fate in vih ΔN egg chambers.

Centrosome migration may be required for
concentrating and confining microtubule nucleation activity to the oocyte in the egg chamber The above result also points to the potential role for the centrosome transport in facilitating the establishment of the oocyte-centric polarized microtubule network within the egg chamber. Thus, we next wished to investigate the possible underlying mechanism through which the transport of germline centrosomes promotes the polarization of the microtubule network. It is known that the microtubule-organizing activity of the centrosome is mediated by the PCM [3,4]. Thus, the PCM may play a role in the formation of the oocyte-centric polarized microtubule network. Therefore, we examined the state of the PCM on germline centrosomes in vih ΔN egg chambers, by staining the Pericentrin-like protein (Plp), a PCM component of both the interphase and mitotic centrosome that is located adjacent to the centriole wall and helps recruit other PCM proteins [3,54]. Consistent with a previous report [23], we observed that Plp labelled centrosomes until late stages of oogenesis in both control and vih ΔN-9 egg chambers. However, in addition to these centrosomal signals, we unexpectedly observed a strong accumulation of Plp on the oocyte nucleus in the control egg chambers, which appeared before S1 and tapered off between S4 and S6 (figure 7d). Although our observation was the first for endogenous Plp proteins, a similar localization pattern on the oocyte nucleus was previously reported for over-expressed GFP-tagged C-terminal domain of Plp (PACT domain) and endogenous γ-tubulin [55][56][57]. We found that, compared to the control, these Plp signals on the oocyte nucleus were significantly reduced in S1-3 vih ΔN-9 egg chambers, which still retained clearly visible membranes between the oocyte and adjacent nurse cells (figure 7d,e). It was previously reported that microtubules also nucleate on the surface of oocyte nuclear membranes and contributes to the posteroanterior movement of the oocyte nucleus in S6-7 egg chambers [55,58]. Thus, the migration of the centrosomes into the oocyte may facilitate a transfer of some pool of PCM to the oocyte nucleus, enabling the oocyte nucleus to act as an MTOC. Such MTOC activity of the oocyte nucleus may contribute to the formation of the robust oocyte-centric polarized microtubule network.
The above observations suggest a potential role of the centrosome transport that promotes the formation of the microtubule network by transferring PCM to the oocyte nucleus. However, this model is somewhat contradictory to the earlier observation made by Stevens et al. [22] using homozygous sas4 mutant flies (note that this study used homozygous sas4 mutants, whereas The quantification of Dynein staining on the oocyte nucleus S1-3 and S4-6 for control and vih ΔN-9 egg chambers with an oocyte nucleus, significance determined using a Welch's unbiased t-test (S1-3: p = 1.4 × 10 −3 ) and a Wilcoxon signedrank test (S4-6 oocyte: 1 × 10 −2 < p < 5 × 10 −1 ). (d) Germaria-S3 and S5 control and vih ΔN-9 egg chambers stained for DNA (DAPI) in blue, PCM (Plp) in green, F-actin (Phalloidin) in red and centrioles (Asl) in white (asterisks indicate oocytes). Scale bars equal to 10 µm. (e) The quantification of Plp staining on the oocyte nucleus S1-3 and S5 control and vih ΔN-9 egg chambers, significance determined using a Wilcoxon signed-rank test (S1-3: 1 × 10 −3 < p < 5 × 10 −3 ; S5: 1 × 10 −2 < p < 5 × 10 −1 ). ( f ) Model for APC/C regulation. APC/C activity needs to be turned off after the last round of germline mitosis in order to stabilize Polo levels thereby enabling the centrosomes to remain stable and be transported to the oocyte. When there is greater APC/C activity then Polo is degraded precociously and the egg chamber becomes destabilized.
royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 the heterozygous sas4 mutation was used in figure 3, keeping one copy of the wild-type sas4 gene) that, in the ovaries where the vast majority of germ cells (approx. 80%) do not have detectable centrosomes, the oocyte develops normally. To reconcile this apparent controversy, we hypothesize that the centrosome transport may facilitate the establishment of the oocyte-centric microtubule network through two functionally redundant processes: first, bringing centrosomes into the oocyte, together with the PCM (figure 7d,e) and, second, removing centrosomes from nurse cells. Centriole loss would affect the first process but not the other. Based on this hypothesis, we next examined ectopic centrosomes that fail to move to the oocyte and remain in nurse cells. We found that Plp signals were also observed on the mislocalized centrosomes in nurse cells both in control and vih ΔN-9 mutant egg chambers (electronic supplementary material, figure S5A). Short microtubule bundles nucleate at ectopic centrosomes in vih ΔN-9 egg chambers (figure 7a). To assess whether mislocalized centrosomes indeed nucleate microtubules, we performed live imaging of egg chambers expressing GFP-fused microtubule plus-end tracking protein EB1 [59] and examined the formation of EB1 comets at individual centrosomes. To avoid pleiotropic effects, we selected S4-5 vih ΔN-9 egg chambers that did not display the membrane phenotype. We observed microtubule nucleation at mislocalized centrosomes in nurse cells in vih ΔN-9 egg chambers, as well as a rare population of mislocalized centrosomes in control egg chambers (electronic supplementary material, figure  S5B and movies S5 and S6). Thus, after being kept inactive during the migration of the centrosomes [21], the activity of the centrosomes appears to be reactivated to start nucleating microtubules ectopically in nurse cells. These ectopic MTOCs, in large numbers, may interfere with the formation of the oocyte-centred microtubule network.
To test a potential adverse effect of microtubule nucleation at ectopic centrosomes, we inhibited microtubule polymerization in vih ΔN-9 mutant egg chambers by feeding flies the microtubule destabilizing drug colcemid. Egg chambers from colcemid-fed flies showed clear patterning defects at later stages both in control and vih ΔN-9 mutant ovaries, however, did not affect centrosome migration, in accordance with previous reports [17,24]. Thus, we could not directly assess the effect of colcemid treatment on the maintenance of oocyte fate (Orb accumulation) in vih ΔN mutant ovaries. Therefore, we examined its effect on the membrane phenotype. We found that, in colcemid-fed vih ΔN-9 mutants, the percentage of egg chambers with the membrane phenotype was partially reduced compared to untreated flies (from 45 to 30%, p = 0.021; electronic supplementary material, figure S5C,D), suggesting the involvement of microtubule nucleation at ectopic centrosome in this phenotype.
Together, these results suggest the critical importance of centrosome migration for oocyte development in two ways: first, to facilitate the formation of oocyte-centric microtubule network and, second, to prevent microtubule nucleation at ectopic nurse cells centrosomes.

Discussion
The intracellular transport of germline centrosomes following cyst formation is observed in diverse animals from insects to mammals, suggesting its functional significance in oogenesis.
However, its exact role, as well as the underlying mechanism directing this event, remains unclear. This is in part due to difficulty specifically manipulating this process without affecting other concurrent events that influence oocyte specification [24,25]. In this present study, by using CRISPRmediated genome editing in Drosophila, we created novel mutants in vih gene, in which the centrosome migration is impeded with the intact fusome formation and proper initial oocyte specification. By using these mutants, we identified a molecular pathway controlling the centrosome transport, shedding a new light into the role of the centrosome migration in oocyte development.
Our study identified an evolutionarily conserved kinase Polo/Plk1 as a key regulator of the centrosome migration in the Drosophila female germline. Polo/Plk1 has been established as a critical regulator of the centrosome in both mitotic and postmitotic cells. Polo/Plk1 recruits PCM components to the centrosome through phosphorylation of centrosome components, which is essential not only for the microtubule nucleation activity of centrosomes but also critical for the stability of centrioles [23,46]. We showed that the expression levels of Polo were significantly decreased in vih ΔN mutant ovaries and that increasing the polo gene dosage fully rescued the centrosome migration defects and the membrane phenotype in vih ΔN mutant germlines (figure 4b-d). Moreover, polo mutant females also exhibited a defect in the centrosome migration as well as the disruption of nurse cell membranes, similar to vih ΔN mutants (figure 4c-g). Together, these results strongly suggest the critical importance of Polo in the regulation of the intercellular migration of centrosomes in the Drosophila female germline (figure 7f ). However, our study could not clarify the downstream molecular events through which Polo directs the centrosome migration, including its direct target required for the migration. Our data suggest that centrioles become destabilized in vih ΔN mutant germlines ( figure 3a,b) and it was recently shown that the local level or activity of Polo at centrioles is a rate-limiting factor for centriole degeneration in the germline cyst/egg [23]. Thus, one plausible model for the role of Polo is that Polo activity may be required to retain PCM on migrating germline centrioles that ensures the structural integrity and physical strength of the centrioles during migration. To support this model, further destabilization of centrioles, by the reduction of a core centriole component Sas4, increased the incidence of centrosome migration failure of vih ΔN-9 mutants (figure 3c-e). Alternatively, as centrosomes migrate along the fusome [17,21], some PCM component recruited by Polo may be directly involved in the interaction between germline centrioles with the fusome. The fusome is decorated with stable acetylated microtubules through the function of the spectraplakin Shot, which is also essential for centrosome migration [25]. The PCM component may directly bind the stable microtubules on the fusome. It is also possible that Polo may regulate centrosome migration independently of the PCM. It was previously shown that, in Drosophila ovaries, Polo binds BicD, a cargo adaptor protein that interacts with the microtubule motor dynein [60]. Further investigation is clearly needed to define the role of Polo in the centrosome transport.
Our study also highlights APC/C, the major ubiquitin ligase in cell cycle control, as an upstream regulator of Polo in its function in centrosome migration (figure 7f ). Polo/ Plk1 has been shown to be an APC/C target in diverse organisms from yeast to humans [48,61]. Our in vivo data and the data from previous in vitro studies on human Vih orthlogue, Ube2C [37,41], suggest that vih ΔN mutations may disrupt negative regulation of APC/C by Vih through the function of its conserved N-terminal extension, which causes precocious or excess Polo degradation in the germline cyst (figure 7f ). The rapid and local control of Polo activity is possibly only achievable by proteolytic degradation; transcriptional regulation of polo mRNA levels would not allow for a rapid alteration of local protein levels. The APC/ C-dependent proteolysis may be critical to fine-tune Polo levels in order to couple the centrosome behaviour to cell cycle regulation in the Drosophila female germline. After the completion of mitotic division of cystoblasts, APC/C activity must be turned off to allow Polo accumulation for the centrosome migration and to maintain a pre-meiotic arrest of the oocyte [62]; it then turns back on to degrade Polo to eliminate centrioles from the oocyte and also to maintain endocycling of nurse cells [23,63] (figure 7f ). Given the conserved roles of the APC/C and Polo kinase, our findings are likely to translate to many other organisms.
Our detailed characterization of the phenotypes in vih ΔN mutant egg chambers suggests a critical role of the centrosome transport in Drosophila oogenesis. Previous studies showed that the activities of dynein and Shot are required for centrosome migration. However, in addition to centrosome migration, dynein mutations also affect the fusome structure and Shot mutations prevent the accumulation of microtubules and Orb in a presumptive oocyte, obscuring the specific role of centrosome migration in oocyte specification [24,25]. In vih ΔN mutant egg chambers, which we created by CRISPR technique, the fusome structure appears normal and Orb, microtubules and specific cell cycle proteins (Dap and CycE) all initially accumulate in the oocyte (figures 6 and 7; electronic supplementary material, figure S3). Thus, in agreement with Stevens et al. [22], these results suggest that the transport of centrosomes is dispensable for oocyte specification. However, to our surprise, we found that the majority of vih ΔN mutant egg chambers eventually lose the oocyte: the oocyte does not retain Orb and becomes polyploid, like nurse cells ( figure 6). We also observed the loss or multiplication of the oocyte in polo 1/11 mutant egg chambers, pointing to a critical role of the centrosome migration in the maintenance of oocyte identity. Although this result may appear contradictory with the results in the aforementioned study [22], it is not. In vih ΔN mutant egg chambers, centrioles are absent (more precisely, reduced) in the oocyte, but, unlike homozygous sas4 mutants, used by the previous study [22], centrioles are abnormally present in nurse cells. Thus, the phenotypes in vih ΔN mutants are the consequences of germline centrosomes being misplaced, not eliminated entirely. Like our observations in vih ΔN mutants, there are indeed many examples in which ectopic centrosomes, not the loss of centrosomes, cause serious consequences, including tumorigenesis, as reported in mice over-expressing Ube2C [38]. Therefore, our results extend beyond the specific role of centrosomes in Drosophila oocyte development to give insight into the roles and underlying mechanism of centrosome regulation across tissues and organisms.
How does centrosome migration control oocyte maintenance? Although our present study cannot provide a definitive answer to this question, our data suggest that the migration of centrosomes into the oocyte may be crucial for the formation of the oocyte-centric polarized microtubule network within the egg chamber, which is considered vital for the maintenance and maturation of the oocyte, mediating directed intercellular trafficking of proteins, RNA and organelles between/within the oocyte and nurse cells. In vih ΔN mutant egg chambers, even those that still retain visible nurse cell-oocyte membranes, we observed reduced accumulation of the minus end-directed microtubule motor dynein in the oocyte, which indicates the weakening of microtubule polarization within the cyst. Interestingly, we observed that an interphase PCM component Plp temporally accumulates on the oocyte nucleus in early-stage egg chambers, which is significantly reduced by vih ΔN mutations (figure 7d,e). It was previously shown that the oocyte contains an MTOC, which nucleates a polarized microtubule network during early stages of oocyte development [17,21]. It was also shown that the oocyte nucleus itself acts as an MTOC after S6 [55,58]. Thus, once centrosomes have reached the oocyte, a fraction of PCM, including Plp, may be transferred from the centrosomes over to the oocyte to confer the oocyte nucleus the microtubule nucleation activity. In addition, we also showed that the centrosomes that fail to reach the oocyte start nucleate microtubules ectopically in nurse cells (figure 7; electronic supplementary material, figure S4B and movies S5 and S6), which if present in a large number, is likely to interfere with proper microtubule organization within the cyst. To support this, we showed that the inhibition of microtubule polymerization by colcemid partially suppresses the membrane phenotype in vih ΔN mutants (electronic supplementary material, figure S5C,D). Thus, centrosome migration may also be important to prevent ectopic microtubule nucleation in nurse cells. Based on these observations, we hypothesize that the intracellular transport of the centrosomes may facilitate the formation of the oocyte-centred microtubule network through the two redundant mechanisms: by efficiently transferring microtubule nucleation activity to the oocyte, and by preventing microtubule nucleation in nurse cells. However, further studies are clearly needed to establish this model and to elucidate the molecular mechanisms underlying the connection between centrosome migration and the formation of the polarized microtubule network in the Drosophila female germline.

Generation of the transgenic vih mutants
The gRNA sequenced used was CGAGCAAAGTGGTG GAGCAG. The target site was selected in order to direct Cas9 cleavage to just after the 5 0 start methionine codon of the transcript. The CRISPR Optimal Target Finder (http:// tools.flycrispr.molbio.wisc.edu/targetFinder/) was used to design the 20mer target sequence. Off-target assessment was done with this program and the target site was chosen because it did not have any homologous sites anywhere else in the genome. The gRNA plasmid pCFD3 (a gift from Fillip Port) was used to create the gRNA transgenic flies [40]. The oligos were cloned directly into the pCFD3 vector for the production of the transgenic gRNA line. All fly embryos were injected by the Cambridge Genetic Fly Facility, using standard procedures. The gRNA expression plasmid was inserted into the genome using the Phi31C system at the attP40 site.
For each experiment, transgenic cas9 virgin females were crossed to U6-gRNA-expressing males carrying the gRNA plasmid insertion, similar to previous studies [40]. Individual females resulting from this cross were subsequently crossed to a balancer stock to remove the Cas9 expression and the resulting single females were again crossed to the balancer stock to generate a stable fly line. Therefore, the other chromosomes that were present during the mutagenesis were eliminated during stock creation. When the alleles were created in an FRT background, the gRNA line was first balanced and crossed to flies containing the FRT chromosome; males of this line were then crossed to transgenic cas9 virgin females and carried through the normal procedure.

CRISPR allele characterization and additional phenotypic data
In order to identify CRISPR/Cas9-induced mutations, genomic DNA was isolated from flies by crushing them in 200 µl of BufferA (100 mM Tris pH 9.0, 100 mM EDTA, 1% SDS), and incubating the lysate at 65-70°C for 30 min. The lysate was chilled on ice for 5 min, before adding 30 µl of 7.5 M NH 4 -acetate. The lysate was then mixed gently, chilled on ice for 20 min and centrifuged for 10 min at 13 000 rpm. The supernatant was transferred to a new tube and spun again for 10 min. The supernatant was again transferred to a new tube, mixed gently with 150 µl of isopropanol and spun again. The supernatant was removed and the DNA pellet was washed with 70% ethanol. The DNA was then dissolved in 100 µl of dH 2 O. One microlitre was used per PCR reaction. PCR was performed with the primers: AAGCCAAA CAGCGGATAGCA and TGGTTGGCAGTAGGTCTTCG. PCR products were gel verified and sent for sequencing. The sequencing of genomic DNA from heterozygous flies yielded an overlay of the DNA sequence from both chromosomes. The mutant sequence was then manually called from the chromatogram. The vih Null alleles have either 1-or 4-nucleotide deletion, resulting in a frame-shift at the 8th amino acid of the gene, which disrupts all domains of the protein. The vih Null alleles were created using different Cas9-expressing lines in different genetic backgrounds. None of these alleles are homozygous viable after larval stage 3, and they do not complement two vih deficiencies nor the vih KG02013 allele [34]. We were able to rescue the viability of the two null alleles with ubiquitously expressed Vih WT and Vih ΔN-9 but we were not able to rescue viability with Vih ΔCS , a catalytically dead version of Vih, and only the transgenically expressed Vih WT allele was able to rescue the fertility (data not shown).
The vih ΔN-9 mutation is a deletion of 9 amino acids in the 27-amino acid N-terminal region. The vih ΔN-9 allele is homozygous viable and complements two vih deficiencies. The other N-terminal allele, vih ΔN allele (vih ΔN-4 ) is a deletion of only 4 amino acids. This allele was created using a different Cas9expressing line directly on an FRT chromosome, and was, therefore, created in a completely different genetic background. Transheterozygous vih ΔN-9 /vih ΔN-4 has the same phenotype as the vih ΔN-4 allele alone and neither alleles have a phenotype when crossed to a vih deficiency (data not shown). The phenotype that was present in both alleles increased with age and an age of 14 days was chosen for analysis, unless otherwise stated. The third chromosome with the vih ΔN-9 allele on it was isogenized after the stock was originally created and rebalanced.

Western blots
For the western blots of Drosophila ovaries, 30 ovaries were dissected in 60 µl of PBS containing Protease and Phosphatase inhibitor (Roche). The samples were lysed using a homogenizing pestle (Sigma-Aldrich), and the lysates were clarified by centrifugation. Two times Laemmli buffer was added to the cleared lysates, and the samples were boiled 2 min. The proteins were then resolved by SDS-PAGE. The electrophoretic run was performed using a Mini-PROTEAN Tetra Cell System (BioRad), in a Running Buffer solution (25 mM Tris, 192 mM glycine and 0.1% SDS, pH approx. 8.6, Sigma), at 200 V. The gel was assembled in a 'transfer sandwich' (cushion pad-filter paper-gel-membrane-filter paper-cushion pad) and blotted on a nitrocellulose membrane (GE Healthcare) for 2 h at 60 V in Transfer Buffer solution (25 mM Tris, 190 mM Glycine, 20% Methanol). Protein transfer was verified by Ponceau S staining, and the membrane was incubated for 45 min at room temperature in a blocking solution containing 5% milk (Marvel) and 0.1% Tween (Sigma) in PBS. The membrane was then incubated in a primary antibody solution prepared in blocking solution for 1 h at room temperature. The membrane was washed three times for 10 min at room temperature with a solution of 0.1% Tween in PBS (PBST) and then incubated in a secondary antibody solution prepared in blocking solution for 1 h at room temperature. The membrane was washed three times with PBST for 10 min at room temperature, incubated with a peroxidase ECL substrate (Pierce), and the proteins were detected by exposing an X-ray film royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 (Fuji). Primary antibodies: Mouse anti-α-tubulin (1 : 1000) Clone DM1A from Sigma, Mouse α-Polo (1 : 500) and Rabbit α-Vih (1 : 500), Glover Lab.

Western blots, destruction assays and ubiquitination assay intensity measurements
The band intensity was calculated using FIJI, a box was drawn over the band and decreased to only include to area of interest, the background was subtracted for each band and normalized to the loading control (α-tubulin). The relative intensity was calculated by dividing by the control.

Egg laying and hatching rate
In large cages, 50 virgin females were mated with equal numbers males and maintained on apple juice agar plates with fresh yeast; the cages were kept at 25°C.

Intensity measurements of fixed samples
For the Plp and Dynein experiments, the egg chamber samples were prepared in parallel and treated the same. The control was analysed first to establish the confocal settings to be used, which remained unaltered for all images acquired, for the channel being directly compared (which was the 488 channel for all experiments). The intensity measurement was taken using FIJI measurement tool. The measurement section chosen for the Plp and Dynein was a circle drawn to the edges of a nucleus at early time points and used for all images as well as for S5/6, and the pixel histogram was checked to only include the signal of interest. Special care was taken to not include the centrosome-associated Plp or Dynein fluorescence in the intensity measurement analysis, since they are closely associated with the oocyte nucleus and germinal vesicles in the control but not vih ΔN-9 egg chambers. Stacks of egg chambers were taken every 1 µm and the brightest single image was chosen for the intensity measurement analysis. The intensity was subtracted for the background in each individual image and the relative intensity was calculated by dividing by the average of the control.

Live sample preparation
After fattening, 14-day aged mated females that were maintained at 25°C for 16-24 h were dissected and their ovaries were short-term live imaged (1 h at room temperature) by dissecting directly in voltelef oil or in PBS with CellMask (incubated for 15 min prior to being transferred to voltelef oil for imaging).

Microtubule nucleation live-imaging sample preparation
Ovaries from flies aged for 14 days were dissected for in vivo preparation as previously described [66,67]. Images were acquired with a ZEISS LSM 880 Airyscan confocal microscope and analysed using ImageJ. In vivo images were obtained at approximately 25°C with a 40×/1.2 numerical aperture (NA) water immersion objective. Single-focal planes were taken every 2 s and processed with proprietary ZEISS' ZEN 2.1 software for Airyscan resolution optimization. We took an unbiased sampling of the centrosomes that satisfied the binary decision of in the oocyte or not. Additionally, the measurements were normalized for filming time with the centrosomes in focus: for the controls, the number of ectopic centrosomes analysed was 17 and the total duration of movies was 56.7 min. The total time of royalsocietypublishing.org/journal/rsob Open Biol. 11: 200371 focused centrosomes was 42.6 min. At this time, the number of comets was 4. Therefore, the nucleation efficiency (how long it takes a two-week-old control centrosome to nucleate 1 microtubule) was 10.65 min. For the vih ΔN-9 egg chambers, the number of ectopic centrosomes analysed was 19 and the total duration of movies was 63.3 min. The total time of focused centrosomes was 47 min. In this time, the number of comets was 2. Therefore, the nucleation efficiency was 23.5 min.

Ubiquitination assay
For the ubiquitination assay, Drosophila APC/C was immuneprecipitated from 2 g of pMTB-Apc4-TAP embryos. The samples were resuspended in 10 ml of ice-cold Buffer A (75 mM HEPES pH7.5, 150 mM KCl, 1.5 mM EGTA, 1.5 mM MgCl2 a, 7.5% glycerol, 0.1% NP40) containing fresh DTT (5 mM) and complete protease inhibitor cocktail (Roche). Embryos were broken using a glass homogenizer and the lysates were cleared by centrifugation at 20 000 rpm for 30 min. The cleared lysates were mixed with preequilibrated Dynabeads (Invitrogen) conjugated with rabbit IgG (MP Biochemicals) and incubated for 2-4 h with gentle rotation. Non-specific bound proteins were removed by six successive washes in Buffer A which contained low salt followed by a final wash with Buffer B (

Destruction assay
The in vitro destruction assay in Xenopus egg extracts was performed as described before [69]. Briefly, 35 S-methioninelabelled substrate proteins were prepared in a coupled in vitro transcription-translation system (Promega) according to the manufacturer's instructions. Cytoplasmic extracts of cytostatic factor (CSF)-arrested Xenopus eggs were prepared following standard procedures. The CSF extracts were first released into interphase by addition of 0.4 mM CaCl 2 and 10 µg ml −1 cycloheximide, and then incubated for 2-4 h at 23°C. Substrates were added to the extracts and the reactions were started by adding 150 ng of purified Xenopus Fzr (gift from Hiro Yamano) to the mixture. Aliquots were collected into 2× Laemmli buffer at 0, 1, 2 and 3 h, boiled for 2 min and resolved by SDS-PAGE.