ABSTRACT
Egg extracts of the African clawed frog Xenopus laevis have provided a cell-free system instrumental in elucidating events of the cell cycle, including mechanisms of spindle assembly. Comparison with extracts from the diploid Western clawed frog, Xenopus tropicalis, which is smaller at the organism, cellular and subcellular levels, has enabled the identification of spindle size scaling factors. We set out to characterize the Marsabit clawed frog, Xenopus borealis, which is intermediate in size between the two species, but more recently diverged in evolution from X. laevis than X. tropicalis. X. borealis eggs were slightly smaller than those of X. laevis, and slightly smaller spindles were assembled in egg extracts. Interestingly, microtubule distribution across the length of the X. borealis spindles differed from both X. laevis and X. tropicalis. Extract mixing experiments revealed common scaling phenomena among Xenopus species, while characterization of spindle factors katanin, TPX2, and Ran indicate that X. borealis spindles possess both X. laevis and X. tropicalis features. Thus, X. borealis egg extract provides a third in vitro system to investigate interspecies scaling and spindle morphometric variation.
INTRODUCTION
In all eukaryotes, cell division requires the spindle, a highly dynamic, self-organizing, microtubule-based apparatus that accurately segregates replicated chromosomes to daughter cells. Spindle microtubules assemble into a bipolar structure that attaches to chromosomes via their kinetochores and aligns them at the metaphase plate so that sister chromatids are oriented toward opposite spindle poles. Although the basic form and composition of the spindle is conserved, spindle structure adapts to changes in cell size and type, and varies dramatically both across and within species (Wühr et al., 2008; Crowder et al., 2015). While many of the molecules and mechanisms that orchestrate spindle assembly have been elucidated, it remains unclear how specific spindle architectures are established, and how this variation impacts spindle function.
Unfertilized eggs of the African clawed frog Xenopus laevis arrested in metaphase of meiosis II by cytostatic factor (CSF) (Masui and Markert, 1971) can be obtained in large quantities. Their fractionation by centrifugation yields a crude cytoplasmic extract that maintains the metaphase arrest and supports spindle assembly around sperm nuclei or chromatin-coated beads (Sawin and Mitchison, 1991; Heald et al., 1996). Remarkably, spindles formed in egg extracts of the smaller, related frog Xenopus tropicalis are shorter in length independent of DNA source, and mixing the two extracts produced spindles of intermediate size (Brown et al., 2007). It was found that compared to X. laevis, X. tropicalis possess smaller spindles due to (i) elevated activity of the hexameric AAA-ATPase microtubule severing enzyme katanin (Loughlin et al., 2010, 2011), and (ii) a higher concentration of the spindle assembly factor, TPX2 (targeting factor for Xklp2), which promotes association of the cross-linking spindle motor Eg5 and a shift of microtubule density from antiparallel overlap in the center of the spindle to the poles (Helmke and Heald, 2014). X. tropicalis spindles were also observed to possess distinct morphological features, including more robust kinetochore fibers and a more circular shape (Loughlin et al., 2011; Grenfell et al., 2016). Furthermore, whereas spindle assembly in X. laevis extracts required a chromatin-generated gradient of RanGTP (Kalab et al., 2002; Cavazza and Vernos, 2016), X. tropicalis spindle assembly was not affected by disruption of this pathway (Helmke and Heald, 2014). Therefore, not only spindle size, but also spindle architecture, morphology, and assembly mechanisms differ between these two species.
To further address the conservation of spindle morphology, assembly, and scaling mechanisms across evolution, we decided to characterize a third Xenopus species, the Marsabit clawed frog Xenopus borealis. Whereas allotetraploid X. laevis (36 chromosomes) and diploid X. tropicalis (20 chromosomes) diverged 48 million years ago, X. borealis is more closely related to X. laevis, having diverged 17 million years ago (Session et al., 2016). Like X. laevis, X. borealis possesses an allotetraploid genome of 36 chromosomes. Interestingly, X. borealis was used extensively in the 1970s to analyze the conservation of ribosomal nucleic acids compared to X. laevis (Brown et al., 1972; Brown and Sugimoto, 1974; Griswold et al., 1974; Leister and Dawid, 1975; Wellauer and Reeder, 1975; Ford and Brown, 1976) and was misidentified as Xenopus mulleri until 1977 (Brown et al., 1977). Revisiting this species and applying the egg extract methodology allowed us to further evaluate spindle morphometric variation and scaling in Xenopus. We show that X. borealis spindles are intermediate in size and display properties of both X. laevis and X. tropicalis, resulting in distinct features. These findings highlight the evolutionary plasticity of spindle morphology and assembly mechanisms, and introduce X. borealis as a third Xenopus species amenable to in vitro assays to investigate the molecular basis of spindle variation.
RESULTS AND DISCUSSION
In this study, we characterized X. borealis and spindle assembly in its egg extracts, using the two well-characterized Xenopus species, X. laevis and X. tropicalis, for comparison.
X. borealis frogs, eggs, and sperm are morphologically distinct
At ∼7 cm body length, adult X. borealis adult frogs were intermediate in size between X. laevis (∼10 cm) and X. tropicalis (∼4 cm) and also displayed distinct physical traits including googly eyes and a pear-like body shape (Figure 1A). Measuring the size of X. borealis gametes revealed that X. borealis eggs averaged 1.2 ± 0.02 mm in diameter, slightly smaller than X. laevis (1.3 ± 0.05 mm) and larger than X. tropicalis (0.75 ± 0.02 mm) (Figure 1B). Interestingly, X. borealis sperm cells were significantly longer (average 22 ± 2.8 μm) than those of both X. laevis (19 ± 2.3 μm) and X. tropicalis (13.5 ± 2.1 μm) (Figure 1C), and similar size differences were observed comparing isolated sperm nuclei (Supplementary Figure S1) (Grainger, 2012). In vitro fertilization and live imaging revealed that the rate of early development of X. borealis and X. laevis embryos were similar (Figure 1D and Video 1) (Nieuwkoop and Faber, 1994). Nuclei isolated from stage 8 (5 hpf) embryos of X. borealis (average 2214 ± 1016 μm2) were comparable in size to those from X. laevis (2010 ± 1081 μm2), while X. tropicalis nuclei (405 ± 116 μm2) were significantly smaller (Figure 1E). In summary, although X. borealis display distinct traits, our measurements show that like X. laevis and X. tropicalis, X. borealis egg size scales with adult animal size, and that X. borealis development and nuclear size is very similar to that of X. laevis. These findings are consistent with the well-characterized phenomenon that genome size scales with nuclear and cell size among amphibians (Levy and Heald, 2016).
X. borealis egg extract recapitulates cell cycle events
To evaluate the utility of X. borealis eggs for in vitro assays, we adapted published ovulation procedures to reproducibly obtain metaphase II, CSF-arrested eggs in sufficient amounts to prepare egg extracts (see Material and Methods). X. borealis eggs were dejellied and fractionated using standard protocols (Hannak and Heald, 2006; Maresca and Heald, 2006; Brown et al., 2007), and produced similar yields of cytoplasmic extract compared to X. laevis despite their smaller body and egg size. X. borealis egg extract was then combined with X. borealis sperm nuclei and assayed for spindle assembly. When added directly to CSF extract, sperm nuclei induced the formation of asters (t = 5’), followed by half-spindles (t = 15’) and bipolar CSF spindles (t = 30 - 45’) (Figure 2A, B). Addition of calcium together with sperm nuclei induced exit from metaphase arrest and formation of interphase nuclei within 45 min. Following the addition of fresh CSF extract, bipolar “cycled” spindles assembled from 75 min to 90 min (Figure 2A, C). We noted that X. borealis extracts formed spindles more quickly than X. laevis, almost as rapidly as X. tropicalis (unpublished data). These experiments show that, as for the other Xenopus species, X. borealis egg extracts are fully capable of recapitulating the cell cycle and assembling spindles in vitro.
Xenopus species possess distinct spindle morphometrics
We next examined some parameters of X. borealis spindle size and microtubule organization and compared them to in vivo meiosis II spindles as well as to spindles assembled in X. laevis and X. tropicalis egg extracts. X. borealis spindles assembled in vitro were similar in length from pole-to-pole and width at the metaphase plate to meiotic spindles imaged in metaphase II-arrested eggs (length/width average 43.9 ± 5.5 μm/21.7 ± 3.6 μm in vivo vs. 44.4 ± 5.5 μm/23.4 ± 5.9 μm in extract) (Figure 3A). X. borealis extract was also capable of inducing bipolar spindle assembly around stage 8 X. borealis embryo nuclei and 10 μm diameter chromatin-coated beads (Halpin et al., 2011). Embryo nuclei spindles were slightly smaller than those formed around sperm nuclei (average length 39.7 ± 4.4 μm, width 25.1 ± 4.7 μm) (Figure 3B), while spindles assembled around DNA-coated beads were considerably shorter (average 22.4 ± 3.9 μm) (Figure 3C). These measurements demonstrate that like X. laevis and X. tropicalis, spindles formed in X. borealis egg extract mimic the size and morphology of the meiotic egg spindle, and that spindle assembly in vitro occurs in the presence or absence of centrosomes.
Despite their smaller egg size, we found that cycled X. borealis spindles were similar in length to X. laevis (average 41.9 ± 4.1 μm vs. 41.6 ± 6.0 μm), but significantly narrower (average 19.7 ± 3.7 μm vs. 22.4 ± 3.6 μm), thereby reducing spindle area and therefore total microtubule content. X. borealis spindles were both longer and wider than X. tropicalis spindles (average 23.2 ± 3.0 μm in length, 10.4 ± 2.6 μm in width) (Figure 4A). Thus, X. borealis spindles scale with egg size and are intermediate in size between those of X. laevis and X. tropicalis. Interestingly, the three species each displayed unique spindle microtubule distributions across the spindle. As previously reported, X. laevis spindles showed a consistent plateau of tubulin intensity along the length of the spindle indicating the presence of an overlapping, tiled array of microtubules (Loughlin et al., 2010). In contrast, X. tropicalis tubulin intensity was greater at the poles and reduced in the center of the spindle at the metaphase plate (Helmke and Heald, 2014). Interestingly, X. borealis spindles displayed a similar increase in microtubule density at the poles as X. tropicalis, a similar density at the metaphase plate as X. laevis, and a unique dip in tubulin intensity between the poles and metaphase plate (Figure 4B). While similar microtubule distribution patterns were observed in CSF spindles, they were less distinct than in cycled spindles, potentially due to the absence of sister kinetochores and associated microtubules (Grenfell et al., 2016). X. borealis CSF spindles were also longer and wider than both X. laevis and X. tropicalis (Supplementary Figure S2). A difference in spindle morphology between spindles with replicated (cycled) and unreplicated (CSF) chromosomes has been observed previously and emphasizes the fact that spindle morphology can vary in different cellular contexts (Grenfell et al., 2016; Levy and Heald, 2016). We decided to focus on cycled spindle assembly for subsequent experiments, as these form around duplicated chromosomes with assembled kinetochores and thus are more physiologically relevant. Therefore, X. borealis fits into the Xenopus interspecies scaling regime, as the animals, eggs and meiotic spindles are all intermediate in size between the other two species. However, X. borealis microtubule arrays share some similarity with both species, leading to a unique spindle architecture.
X. borealis spindles are sensitive to perturbation of the RanGTP gradient
To compare spindle assembly mechanisms among the three species, we examined the role of the RanGTP gradient, which acts to release nuclear localization signal (NLS)-containing spindle assembly factors from importins near mitotic chromatin where the guanine nucleotide exchange factor RCC1 (Regulator of Chromosome Condensation 1) is localized, thereby promoting microtubule nucleation, stabilization, and crosslinking (Cavazza and Vernos, 2016). Perturbing the RanGTP gradient by the addition of Ran mutants, such as a dominant negative (T24N) or constitutively active, GTP-bound (Q69L) form, is detrimental to X. laevis spindle assembly, abolishing it completely or increasing ectopic microtubule nucleation and formation of multipolar spindles, respectively (Kalab et al., 1999, 2002). In contrast, we showed previously that X. tropicalis spindles are much less affected by perturbation of the RanGTP gradient (Helmke and Heald, 2014). To test the role of this pathway in X. borealis, we added the Ran mutants at the onset of spindle assembly. Upon addition of RanT24N, spindle assembly was strongly impaired, with dramatically reduced microtubule nucleation around sperm nuclei, while RanQ69L increased the number of multipolar spindle structures (Figure 5 and Supplementary Table 1). Thus, like X. laevis, X. borealis bipolar spindle assembly depends on the RanGTP gradient.
Common spindle scaling mechanisms operate among Xenopus species
It has been shown that hybrid embryos can be generated by fertilization of X. borealis eggs with sperm from either X. laevis and X. tropicalis (De Robertis and Black, 1979; Gibeaux et al., 2018), indicating compatibility between the X. borealis cytoplasm and the chromosomes of both species. Addition of either X. laevis or X. tropicalis sperm nuclei to X. borealis extract did not alter spindle microtubule distribution (Supplementary Figure S3A), consistent with previous studies indicating that egg cytoplasm composition is the primary determinant of spindle morphology (Brown et al., 2007). To determine whether maternal cytoplasmic factors affect spindle size similarly among the three Xenopus species, we mixed X. borealis egg extract with either X. laevis or X. tropicalis extract in the presence of X. laevis or X. tropicalis sperm nuclei, respectively. Whereas titration of X. borealis extract with X. laevis did not affect spindle dimensions (Figure 6A), X. tropicalis extract caused X. borealis spindles to shrink proportionately with the amount added (Figure 6B). Analysis of spindle microtubule distributions in mixed extracts revealed that these were also affected proportionately, favoring the tubulin distribution of the more abundant extract (Supplementary Figure S3B and C). These results are consistent with cytoplasmic mixing of X. laevis with X. tropicalis extracts, which also caused spindle shrinkage in a dose-dependent manner (Brown et al., 2007). Altogether, these data indicate that common scaling and microtubule organization mechanisms operate among the three Xenopus species.
X. borealis spindles combine scaling factor features of both X. laevis and X. tropicalis
To investigate the molecular basis of X. borealis spindle size and morphology, we compared the localization, abundance, and sequence of katanin and TPX2, two spindle scaling factors that contribute to spindle size differences between X. laevis and X. tropicalis, as well as the microtubule polymerase XMAP215, levels of which have been shown to regulate spindle length in Xenopus (Reber et al., 2013). XMAP215 levels and localization were similar for all three Xenopus species (Supplementary Figure S4). Katanin, a microtubule severing AAA-ATPase, has higher activity in X. tropicalis due to the absence of an inhibitory phosphorylation site (Serine 131) found in the X. laevis protein (Loughlin et al., 2011). Immunofluorescence and line scan analysis of spindles revealed that katanin localization on the X. borealis spindle displays a small but distinct increase at the metaphase plate as well as the spindle poles, while the localization on X. laevis spindles is more uniform and X. tropicalis shows katanin enrichment solely at the poles (Figure 7A). By Western blot, katanin levels did not differ significantly across the three species (Figure 7B). Although the amino acid sequence of X. borealis katanin is over 97% identical to that of both X. tropicalis and X. laevis, it contains the key inhibitory serine residue that regulates katanin activity (Supplementary Figure S5). TPX2 is a Ran-regulated microtubule-associated protein that is found at three-fold higher concentrations in X. tropicalis compared to X. laevis. Increasing the level of TPX2 in X. laevis extracts to that of X. tropicalis was previously shown to reduce spindle length through its increased recruitment of the spindle motor Eg5 to spindle poles (Helmke and Heald, 2014). Interestingly, X. borealis spindles displayed an overall TPX2 localization more similar to X. tropicalis, with higher intensity at the spindle poles, but also possessed a central smaller peak of TPX2 reminiscent of X. laevis (Figure 7C). Levels of TPX2 in X. borealis egg extracts were two-fold higher than in X. laevis, but not elevated to X. tropicalis levels. (Figure 7D). Notably, the amino acid sequence of X. borealis TPX2 is more similar to X. laevis compared to X. tropicalis and contains the seven amino acid residues thought to reduce microtubule nucleation activity of X. laevis TPX2 (Supplementary Figure S6) (Helmke and Heald, 2014; Grenfell et al., 2016). Altogether, these results suggest that X. borealis spindle length results from its lower katanin activity similar to X. laevis, while its microtubule distribution is likely affected by increased levels of TPX2, which is more reminiscent of X. tropicalis.
Overall, these observations reveal that X. borealis meiotic spindles, although more similar in size and RanGTP-dependence to X. laevis, also possess some structural and molecular features characteristic of X. tropicalis. These findings support the idea that katanin and TPX2 are important spindle scaling and assembly factors in Xenopus. Katanin-mediated microtubule severing activity has been shown to regulate spindle size in several organisms, including Caenorhabditis elegans, Xenopus, and human cells (McNally et al., 2006; Loughlin et al., 2011; Joly et al., 2016; Jiang et al., 2017), which is consistent with results from meiotic spindle assembly simulations showing that altering microtubule depolymerization rates robustly scales spindle length (Loughlin et al., 2010).
The role of TPX2 in spindle assembly and size control is more complicated. Depletion of the TPX2 ortholog D-TPX2 from Drosophila melanogaster syncytial embryos and S2 cells resulted in spindle shortening (Goshima, 2011; Hayward and Wakefield, 2014), and human cells require phosphorylation of TPX2 by Aurora A for normal spindle length (Fu et al., 2015). In contrast, addition of recombinant TPX2 to X. laevis extracts decreased spindle length (Helmke and Heald, 2014), and we have observed similar effects on X. borealis spindles (unpublished data). Spindle-shrinking effects in Xenopus did not depend on Aurora A, but rather on a change in spindle microtubule distribution caused by increased recruitment of the cross-linking Eg5 motor to spindle poles (Helmke and Heald, 2014). TPX2 also regulates microtubule nucleation in the spindle (Petry et al., 2013; Scrofani et al., 2015; Petry, 2016; Alfaro-Aco et al., 2017). TPX2 has thus emerged as a central player of spindle assembly and organization in a wide variety of cell types (Ma et al., 2011; Helmke et al., 2013; Fu et al., 2015; Levy and Heald, 2016) and is overexpressed in many cancers (Chang et al., 2012; Neumayer et al., 2014). Our results highlight the importance of TPX2 levels and localization as determinants of meiotic spindle microtubule architecture. TPX2 localization (Figure 7C) correlates well with the distribution of tubulin intensity across all three species (Figure 4B), particularly at the spindle poles (Ma et al., 2011; Helmke and Heald, 2014). Despite having higher TPX2 levels, the greater sequence similarity of X. borealis TPX2 to the X. laevis protein (Supplementary Figure S6) may explain the increased sensitivity to Ran inhibition in X. borealis (Figure 5C), since a 7 amino acid sequence shown to decrease microtubule nucleation activity relative to X. tropicalis is present in both X. borealis and X. laevis TPX2 (Figure 7D) (Helmke and Heald, 2014). Altogether, our results provide clues to how TPX2 levels may tune meiotic spindle architecture and assembly pathways by altering microtubule nucleation and organization.
In summary, Xenopus borealis provides a robust in vitro egg extract that adds to the characterized X. laevis and X. tropicalis systems, enabling further investigation of spindle assembly and interspecies scaling. Our findings highlight that egg meiosis II spindle architecture varies across Xenopus species and suggest that X. borealis spindles assemble with a combination of X. laevis as well as X. tropicalis features.
MATERIALS AND METHODS
Chemicals
Unless otherwise stated, all chemicals were purchased from Sigma-Aldrich, St. Louis, MO.
Frog care
All animal experimentation is this study was performed according to our Animal Use Protocol approved by the UC Berkeley Animal Care and Use Committee. Mature X. laevis, X. tropicalis, and X. borealis frogs were obtained from NASCO, WI. X. laevis, X. tropicalis, and X. borealis females were ovulated with no harm to the animals with a 6-, 3-, and 4-month rest interval, respectively. To obtain testes, males were euthanized by over-anesthesia through immersion in ddH2O containing 0.15% MS222 (Tricaine) neutralized with 5 mM sodium bicarbonate prior to dissection, and then frozen at -20°C.
Sperm nuclei purification
X. laevis and X. tropicalis sperm nuclei were prepared and purified as previously described (Grainger, 2012). The following modifications were made for X. borealis sperm nuclei purification. X. borealis males were primed with 40 U of PMSG 3 days prior to dissection and boosted with 100 U hCG 12-24 h before dissection. Testes were removed and cleaned from all blood vessels and fat with forceps. Testes were then washed 3X in cold 1X MMR (1X MMR: 100 mM NaCl, 2 mM KCl, 2 mM CaCl2, 1 mM MgCl2 and 5 mM HEPES-NaOH pH 7.6, 0.1 mM EDTA) and 3X in cold Nuclear Preparation Buffer (NPB) (2X NPB: 500 mM sucrose, 30 mM HEPES, 1 mM spermidine trihydrochloride, 0.4 mM spermine tetrahydrochloride, 2 mM dithiothreitol, 2 mM EDTA) and placed in 1 mL of cold NPB for homogenization with scissors and a pestle. Samples were briefly spun to pellet the remaining tissue before transferring the supernatant to a new tube for centrifugation at 1500 g for 10 min at 4°C to pellet sperm. The pellet was resuspended in 1 mL NPB supplemented with 50 μL of 10 mg/mL lysolecithin and incubated for 5 min at RT. The resuspended pellet was then added to 4 mL of cold NPB supplemented with 3% BSA and spun at 3,000 RPM for 10 min at 4°C. The resulting pellet was resuspended in 2 mL of cold NPB with 0.3% bovine serum albumin (BSA) and 30% filtered glycerol. Finally, the pellet was resuspended in 500 μL of cold NPB with 0.3% BSA and 30% filtered glycerol. Sperm nuclei were adjusted to a concentration of 108 nuclei per mL using cold NPB with 0.3% BSA and 30% glycerol to make a 200X stock, aliquoted, frozen in liquid nitrogen, and stored at -80°C.
In vitro fertilization
X. borealis males were injected with 300 U of human chorionic gonadotropin hormone (hCG) 12-24 h before dissection and testes were collected in Leibovitz L-15 Medium (Gibco – Thermo Fisher Scientific, Waltham, MA) supplemented with 10% Fetal Bovine Serum (FBS; Gibco) for immediate use. X. laevis males were injected with 500 U of hCG 12-24 h before dissection and testes were stored at 4°C in 1X MR (100 mM NaCl, 1.8 mM KCl, 2 mM CaCl2, 1 mM MgCl2 and 5 mM HEPES-NaOH pH 7.6) for 1-2 weeks.
X. borealis and X. laevis females were primed with 60 U and 100 U, respectively, of pregnant mare serum gonadotrophin (PMSG, National Hormone and Peptide Program, Torrance, CA) at least 48 h before use and boosted with 300 U and 500 U, respectively, of hCG 12-24 h before the experiment. X. borealis and X. laevis frogs were kept at 16°C in 0.5X and 1X MMR, respectively. X. borealis eggs were picked from the tub and deposited onto petri dishes coated with 1.5% agarose in 1/10X MMR. X. laevis females were squeezed gently to deposit eggs onto petri dishes coated with 1.5% agarose in 1/10X MMR. Two X. borealis testes or 2/3 of an X. laevis testis were collected and homogenized using scissors and a pestle in 1 mL of L-15 and 10% FBS. Any excess liquid in the petri dishes was removed, and the eggs were fertilized with 500 μL of sperm solution per dish. Eggs were swirled in the solution to individualize eggs as much as possible and incubated for 5 min. Dishes were flooded with ddH2O, swirled and incubated for 10 min, followed by buffer exchange to 1/10X MMR and incubation for 10 min. The embryo jelly coats were then removed with a 3% cysteine solution in ddH2O-NaOH, pH 7.8. After extensive washing (>4X) with 1/10X MMR, embryos were incubated at 23°C. At stage 2-3, fertilized embryos were sorted and placed in fresh 1/10X MMR in new petri dishes coated with 1.5% agarose in 1/10X MMR.
All embryos were staged according to Nieuwkoop and Faber (Nieuwkoop and Faber, 1994).
Embryo video imaging
Imaging dishes were prepared using a homemade PDMS mold designed to print a pattern of 1 mm large wells in agarose that allowed us to image 4 X. borealis or X. laevis embryos simultaneously within the 3X4 mm camera field of view for each condition. Embryos were imaged from stage 2-3. Videos were taken simultaneously using two AmScope MD200 USB cameras (AmScope, Irvine, CA) each mounted on an AmScope SE305R stereoscope. Time lapse movies were acquired at a frequency of 1 frame every 10 s for 20 h and saved as Motion JPEG using a MATLAB (The MathWorks, Inc., Natick, MA) script. Movie post-processing (cropping, concatenation, resizing, addition of scale bar) was done using MATLAB and Fiji (Schindelin et al., 2012). All MATLAB scripts written for this study are available upon request. Two of the scripts used here were obtained through the MATLAB Central File Exchange: “videoMultiCrop” and “concatVideo2D” by Nikolay S.
Embryo nuclei purification
Following in vitro fertilization, X. borealis embryos were arrested at stage 8 (∼5 hpf) in late interphase using 150 μg/mL cycloheximide in 1/10X MMR for 60 min. Embryos were washed several times in Egg Lysis Buffer (ELB; 250 mM sucrose, 50 mM KCl, 2.5 mM MgCl2, and 10 mM HEPES pH 7.8) supplemented with LPC (10 μg/mL each leupeptin, pepstatin, chymostatin), cytochalasin D (100 μg/mL), and cycloheximide (100 μg/mL), packed in a tabletop centrifuge at 200 g for 1 min, crushed with a pestle, and centrifuged at 10,000 g for 10 min at 16°C. The cytoplasmic extract containing endogenous embryonic nuclei was collected, supplemented with 8% glycerol, aliquoted, frozen in liquid nitrogen, and stored at -80°C.
X. borealis egg extract
X. borealis metaphase-arrested egg extracts were prepared similarly to X. laevis and X. tropicalis (Maresca and Heald, 2006; Brown et al., 2007), with the following modifications. X. borealis female frogs were primed with 60 U PMSG at least 48 hours before use and boosted with 300 U hCG 12-24 hours before the experiment. Frogs were kept at 16°C in 0.5X MMR. The eggs were dejellied in a 3% cysteine solution in 1X XB-salts (20X: 2M KCl, 20 mM MgCl2, 2 mM CaCl2), pH 7.8, and washed in CSF-XB (100 mM KCl, 0.1 mM CaCl2, 3 mM MgCl2, 50 mM sucrose, 10 mM K-EGTA, 10 mM K-HEPES, pH 7.8). CSF-XB buffer was exchanged for CSF-XB supplemented with LPC (10 μg/mL) (CSF-XB+). 1 mL of CSF-XB+ supplemented with cytochalasin D (100 μg/mL) was added to the bottom of an ultracentrifuge tube (SW-55, Beckman) before loading eggs into the tube. Extract tubes were placed in adapter tubes and spun at 1600 g for 1 min to pack the eggs. The excess liquid was removed and the eggs crushed by centrifugation at 10,200 rpm for 16 min at 16°C. The cytoplasmic fraction was then removed and supplemented with LPC (1:1000 dilution; 10 mg/mL stock), cytochalasin D (1:500 dilution; 10 mg/mL stock), energy (1:50 dilution; 50X stock: 190 mM creatine phosphate, 25 mM adenosine triphosphate, 25 mM MgCl2, 2.5 mM K-EGTA pH 7.7), and rhodamine-tubulin (1:300 dilution; 65.8 μg/uL stock) for spindle assembly reactions. Sperm nuclei, embryo nuclei, or 10 μm chromatin-coated beads, prepared as previously described (Halpin et al., 2011), were used as a source of DNA for spindle assembly.
X. laevis and X. tropicalis egg extracts and mixing experiments
X. laevis and X. tropicalis metaphase arrested egg extracts were prepared and spindle reactions conducted as previously described (Maresca and Heald, 2006; Brown et al., 2007). X. laevis or X. tropicalis extracts were mixed in different proportions to X. borealis extract and supplemented with either X. laevis or X. tropicalis sperm nuclei, respectively.
Extract treatments
To examine sensitivity to perturbations of the RanGTP gradient, X. laevis, X. tropicalis, and X. borealis sperm nuclei were added to their respective egg extracts and cycled through interphase. Ran T24N (final concentration 1 μM) and Q69L (final concentration 5 μM) mutant proteins, purified as previously described (Helmke and Heald, 2014), were added to the interphase extract reaction when fresh CSF extract was added to induce the extract to cycle back to mitosis.
Spindle spin-down and immunofluorescence
Spindle reactions were prepared, spun-down, and processed for immunofluorescence as previously described (Hannak and Heald, 2006). Briefly, the extract reactions were fixed for 5-10 minutes with 2.5% formaldehyde and spun down at 10,200 rpm for 16 min at 16°C. The coverslips were incubated for 30 s in cold methanol, washed in PBS+NP40, and blocked overnight in PBS + 5% BSA at 4°C. The anti-TPX2 (1:150 dilution, unpublished), anti-katanin p60 (1:500 dilution) (Loughlin et al., 2011), or anti-XMAP215 (1:200, Tony Hyman & Kazu Kinoshita) rabbit antibodies were added for 1 h in PBS + 5% BSA. After washing with PBS+NP40, the coverslips were incubated with 1:1000 anti-rabbit antibody coupled to Alexa Fluor 488 (Invitrogen – Thermo Fisher Scientific, Waltham, MA) for 30 min and then with 1:1000 Hoechst for 5 min. The coverslips were then washed and mounted for imaging with Vectashield (Vector Laboratories, Burlingame, CA).
Egg whole mount immunofluorescence
Metaphase-arrested X. borealis eggs were fixed for 1-3 h at RT using MAD fixative (2 parts of methanol (Thermo Fisher Scientific, Waltham, MA), 2 parts of acetone (Thermo Fisher Scientific, Waltham, MA), 1 part of DMSO), and stored overnight at -20°C in fresh MAD fixative. Embryos were then processed as previously described (Lee et al., 2008) with some modifications. Following gradual rehydration in 0.5X SSC (1X SSC: 150 mM NaCl, 15 mM Na citrate, pH 7.0), embryos were bleached with 2% H2O2 (Thermo Fisher Scientific, Waltham, MA) in 0.5X SSC containing 5% formamide for 2-3 h under light, then washed in PBT, a PBS solution containing 0.1% Triton X-100 (Thermo Fisher Scientific, Waltham, MA) and 2 mg/ml BSA. Embryos were blocked in PBT supplemented with 10% goat serum (Gibco – Thermo Fisher Scientific, Waltham, MA) and 5% DMSO for 1-3 h and incubated overnight at 4°C in PBT supplemented with 10% goat serum and the primary antibodies. We used the following antibodies: 1:500 mouse anti-beta tubulin (E7; Developmental Studies Hybridoma Bank, Iowa City, IA), 1:350 rabbit anti-histone H3 (ab1791; Abcam, Cambridge, MA). Embryos were then washed 4 X 2 h in PBT and incubated overnight in PBT supplemented with 1:500 goat anti-mouse secondary antibody coupled to Alexa Fluor 488 and 1:500 goat anti-rabbit secondary antibody coupled to Alexa Fluor 568 (Invitrogen – Thermo Fisher Scientific, Waltham, MA). Embryos were then washed 4 X 2 h in PBT and gradually dehydrated in methanol. Embryos were finally cleared in Murray’s clearing medium (2 parts of Benzyl Benzoate, 1 part of Benzyl Alcohol). Embryos were placed in a chamber made using a flat nylon washer (Grainger, Lake Forest, IL) attached with nail polish (Sally Hansen, New York, NY) to a slide and covered by a coverslip, and filled with Murray’s clearing medium for confocal microscopy.
Confocal microscopy
Confocal microscopy was performed on an upright Zeiss LSM 780 NLO AxioExaminer using the Zeiss Zen software. Embryos were illuminated with an LED light source (X-cite 120LED). For the imaging of histone H3 and tubulin, embryos were imaged using a Plan-Apochromat 20x/1.0 Water objective and laser powers of 12%, on multiple 1024x1024 px plans spaced of 0.683 μm in Z. Images are mean averages of 2 scans with a depth of 16 bits. Channels were acquired simultaneously, and pinhole size was always chosen to correspond to 1 airy unit.
Imaging and quantification
Eggs were imaged using the Leica Application Suite (v4.9; Leica Microsystems, Buffalo Grove, IL) with a Wild M7A stereoscope equipped with a Leica MC170HD camera. Sperm cells, sperm nuclei, embryo nuclei, and spindles were imaged using micromanager software (Edelstein et al., 2014) with an Olympus BX51 microscope equipped with an ORCA-ER camera (Hamamatsu Photonics, Hamamatsu city, Japan), and with an Olympus UPlan FL 40x/0.75 air objective. All measurements were made using Fiji. The spindle tubulin, katanin, TPX2, and XMAP215 intensity line scans were measured using an automated Java ImageJ plugin developed by Xiao Zhou (Heald lab, UC Berkeley; https://github.com/XiaoMutt/AiSpindle).
Western blot and analysis
1 μL of egg extract for 3 independent extracts for each species was subjected to SDS-PAGE (12% gel for katanin, 8% gel for TPX2 and XMAP215) and transferred to a nitrocellulose membrane. The anti-TPX2 (1:500 dilution, unpublished), anti-katanin p60 (1:1000 dilution) (Loughlin et al., 2011), or anti-XMAP215 (1:1000, Tony Hyman & Kazu Kinoshita) rabbit antibodies and anti-Ran (1:2000 dilution, BD Biosciences, San Jose, CA) mouse antibody were added for 1 h or overnight at 4°C in PBS + 0.1% Tween-20 + 5% milk. Secondary antibodies (goat anti-rabbit IRDye 800 or goat anti-mouse IRDye 680) were added at 1:10,000 for 1 h in PBS + 0.1% Tween-20. Blots were scanned with an Odyssey Infrared Imaging System (LI-COR Biosciences), and band intensity was quantified with Fiji.
Protein sequence alignments
Multiple sequence alignments were performed using Clustal Omega (default parameters). Sequence similarities were determined by pairwise alignments using EMBOSS Needle (default parameters).
AUTHOR CONTRIBUTIONS
M.K. performed the experiments and analyzed the data, with help from R.G. M.K. prepared the figures and wrote the manuscript with input from R.H. and R.G.
AUTHOR INFORMATION
The authors declare no competing financial interests. Correspondence should be addressed to R.G. (romain.gibeaux@univ-rennes1.fr) and R.H. (bheald@berkeley.edu).
ACKNOWLEDGEMENTS
We thank members of the Heald lab for support and fruitful discussions, in particular Xiao Zhou for his line scan plugin and Ambika Nadkarni for the purification of Ran mutants. We thank Sofia Medina-Ruiz, Austin Mudd, and Dan Rokhsar for providing early access to X. borealis katanin, TPX2, and XMAP215 sequences. The confocal microscopy performed in this work was done at the UC Berkeley CRL Molecular Imaging Center, supported by NSF DBI-1041078. MK was supported by the UC Berkeley MCB department NIH training grant 4T32GM007232-40. RH was supported by NIH R35 GM118183 and the Flora Lamson Hewlett Chair. RG was supported by an HFSP long term fellowship LT 0004252014-L.