Abstract
At the onset of meiosis, each chromosome needs to find its homologue and pair to ensure proper segregation. In Drosophila, pairing occurs during the mitotic cycles preceding meiosis. Here we show that germ cell nuclei undergo marked movements during this developmental window. We demonstrate that microtubules and Dynein are driving nuclear rotations and are required for centromere pairing and clustering. We further found that Klaroid (SUN) and Klarsicht (KASH) co-localize with centromeres at the nuclear envelope and are required for proper chromosome motions and pairing. We identified Mud (NuMA in vertebrates) as co-localizing with centromeres, Klarsicht and Klaroid. Mud is also required to maintain the integrity of the nuclear envelope and for the correct assembly of the synaptonemal complex. Our findings reveal a mechanism for chromosome pairing in Drosophila, and indicate that microtubules, centrosomes and associated proteins play a crucial role in the dynamic organization of chromosomes inside the nucleus.
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Acknowledgements
We wish to thank F. Llense for observing that Mud co-localized with centromeres and E. Heard for suggesting ‘rolling’ nuclei. We are grateful to S. Roth (University of Cologne, Germany), M. Welte, J. Fischer and the Bloomington Stock centre for flies and reagents. We acknowledge great technical support from the PICT@BDD imaging platform. This work was supported by the European Research Council (ERC EPIGENETIX No 250367). N.C. is supported by Institut Curie, FRM post-doctoral fellowship (SPF20111223331) and DEEP LabEx; T.R. is supported by an FRM Ingenieur Fellowship (no ING20140129247); the J.-R.H. laboratory is funded by CNRS, Ville de Paris, ANR and FSER (Schlumberger).
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N.C., T.R. and J.-R.H conceived and designed the experiments. N.C., T.R. and M.A. performed the experiments. N.C., T.R. and J.-R.H. analysed the data. I.B. conceived and performed centromere correlation analysis. T.P. performed SIM microscopy. J.-R.H. and N.C. wrote the paper.
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Integrated supplementary information
Supplementary Figure 1
(A) Mean nuclear volume for each cell stage in region 1 in Nup::GFP/+; CID::RFP/+ living germarium. For each nucleus, its longest diameter (D) and its smallest diameter (d) were determined by measuring the distance between two diametrically opposed Nup::GFP signals on projected images along the x–y axis. The height of the nucleus (h) was determined on z-series that range from the first Nup foci until the last Nup foci seen. The volume (μm3) was calculated using the formula: V = 4 × D × d × h × π/3. The number of analyzed nuclei (n value) is indicated under each stage. Centre and error bars are mean ± SD. (B) The coordinated motion between centromeres doublets at stem cell and 8cc stages. Distances between centromeres were measured in 3D time-lapse images (SC, n = 41; 8cc, n = 52). On the basis of the following criteria, centromere doublets were classified according to their attachment coefficient. Only doublets displaying 15 common time points and with a correlation coefficient < 0.95 were taken into account for calculation of the attachment coefficient. 25% of centromere doublets display an attachment coefficient superior to 0.75 (red line) at 8cc stage (blue bars), whereas none of centromere doublets reach this value at stem cell stage (grey bars). GSC: n = 49 pairs of tracks having more than 15 common time-points and correlation coefficient smaller than 0.75. 8cc: n = 39 pairs of tracks having more than 15 common time-points and correlation coefficient smaller than 0.95).
Supplementary Figure 2
(A) Inactivation by UV of the microtubule inhibitor colcemid does not affect CID foci dynamics in stem cells. Selected projections of Z-sections of single stem cells are shown. In the first two projections colcemid is active, microtubules are depolymerized and centromeric foci movement is very limited. In the last three projections colcemid was inactivated with a 5 s UV pulse and centromeric movement is not altered. For each time point, the cumulative tracking is represented in the bottom half picture. The yellow and white dotted circles indicate the nuclear surface of two nuclei in each image. (B,B’) 3D representations indicating the covered volume of the selected representative track corresponding to the yellow nucleus for all time points, the ellipsoid is arbitrarily centered into a sphere representing the nuclear volume of the stem cell nucleus before the UV pulse (B) and the same 8cc after UV pulse (B’).
Supplementary Figure 3 Developmental changes in the number of CID foci in region 2a and 2b in fixed germarium.
For each genotype, the mean number of CID foci in region 2a (blue bars) and in region 2b (red bars) is indicated. ∗P < 0.05 (data collected across 3 independent experiments for each genotype; centre and error bars are mean ± S.D). wt region 2a n = 89 nuclei from 13 germarium; wt region 2b n = 55 from 21 germarium; nos>Dhc-shRNAi region 2a n = 75 nuclei from 5 germarium; Dhc64c3−2/Dhc64c6−12 region 2a n = 224 nuclei from 6 germarium; wt+ colcemid region 2a n = 49 nuclei from 13 germarium; wt + colcemid in region 2b n = 24 nuclei from 13 germarium; Sas4s2214 region 2a n = 68 from 23 germarium; Sas4s2214 region 2b n = 23 from 14 germarium; AslMecD region 2a n = 52 nuclei from 12 germarium; AslMecD region 2b n = 21 from 12 germarium; Sas4-RNAi region 2a n = 78 from 12 germarium; Sas4-RNai region 2b n = 22 from 11 germarium; asl-RNAi region 2a n = 96 from 12 germarium; asl-RNAi region 2b n = 22 from 12 germarium; klarmarbCD4 region 2a n = 102 nuclei from 13 germarium; klarmarbCD4 region 2b n = 45 from 30 germarium; koi80 region 2a n = 71 nuclei from 13 germarium; koi80 region 2b n = 47 from 29 germarium; klarmarbCD4;koi80 region 2a n = 199 nuclei from 21 germarium; klarmarbCD4;koi80 region 2b n = 46 nuclei from 28 germarium; klar-RNAi region 2a n = 70 nuclei from 7 gerrmaria; klar-RNAi region 2b n = 21 nuclei from 11 germarium; koi-RNAi region 2a n = 79 nuclei from 10 germarium; koi-RNAi region 2b n = 29 from 16 germarium; mudfO1205 region 2a n = 131 nuclei from 15 germarium; mudfO1205 region 2b n = 45 nuclei from 28 germarium; mud-RNAi (Bl:35044) region 2a n = 62 nuclei from 6 germarium; mud-RNAi (Bl:35044) region 2b n = 17 nuclei from 12 germarium; mud-RNAi (Bl:38190) region 2a n = 51 nuclei from 6 germarium; mud-RNAi (Bl:38190) region 2b n = 13 nuclei from 9 germarium; klarmbCD4/+ region 2a n = 81 nuclei from 18 germarium; klarmbCD4/+ region 2b n = 34 nuclei from 22 germarium; koi80/+ region 2a n = 87 nuclei from 18 germarium; koi80/+ region 2b n = 36 nuclei from 19 germarium; mudfO1205; klarmbCD4/+ region 2a n = 257 nuclei from 40 germarium; mudfO1205; klarmbCD4/+ region 2b n = 59 nuclei from 38 germarium; mudfO1205; koi80/+ region 2a n = 86 nuclei from 19 germarium; mudfO1205; koi80/+ region 2b n = 41 nuclei from 26 germarium.
Supplementary Figure 4
Projections of Z-sections obtained by DV microscopy of a wild-type stem cell nucleus (Aa–Ac), a 4-cell cyst nucleus (Ba–Bc), an 8-cell cyst nucleus (Ca–Cc), a 16-cell cyst nucleus (Da–Dc) and a stage 3 ovocyte nucleus (Ea–Ec) stained for centromere (CID, orange), Klarsicht (Klar, green), Klaroid (Koi, magenta) and DNA (DAPI, blue). Koi and klar display a perinuclear localization in SCs and stage3 ovocytes (A,E). In some 4-cell cysts and 16-cell cysts koi and klar localize as dots at the nuclear membrane (B,D). In 8-cell cysts koi and klar localize as dots at the nuclear membrane.
Supplementary Figure 5
(A,B) 3D representations indicating the relative covered volume of one selected representative track for all time points of a CID::RFP;nos/klar-shRNA (A), and a CID::RFP, nos/koi-shRNA (B) 8cc selected nucleus. The ellipsoid is arbitrarily centered into a sphere representing the nuclear volume (gold sphere). (C) Distributions of the relative covered volume per second for centromeric foci in CID::RFP;w-shRNA, CID::RFP;nos/klar-shRNA, and CID::RFP, nos/koi-shRNA 8cc nuclei (mean ± S.D. Mann–Whitney U-test comparing CID::RFP;w-shRNA with CID::RFP;nos/klar-shRNA: p ≤ 1 × 10−4 and with CID::RFP, nos/koi-shRNA: p = 0.1622). nos>w-shRNA = 44 centromeric foci/4 experiments; nos>klar-shRNA = 94 centromeric foci/6 experiments; nos>koi-shRNA = 43 centromeric foci/4 experiments.
Supplementary Figure 6 Changes in the percentages of germarium displaying Polycomplexes in wild-type, koi80; klarmarb−CD4, mudf01205, nos>mud-shRNA38190 and nos>mud-shRNA35044.
The number of analyzed germarium is indicated under each stage.
Supplementary Figure 7
(A) Changes in the percentage of germarium displaying SC defects in wild-type, klarmarb−CD4, koi80, koi80; klarmarb−CD4 and mudf01205 and their respective sh-RNAs (in all cases except koi80 and koi-shRNA khi2 < 0.0005). The number of analyzed germarium is indicated for each stage. wt n = 145 germarium collected across 3 independent preparations; mudf01205n = 280 germarium; 3 independent preparations; mud-RNai (Bl:38190) n = 88; 3 independent preparations; mud-RNAi (Bl:35044) n = 98; 3 independent preparations (B) SC fluorescence intensity was quantified in all mutant and sh-RNA conditions. Each one was normalized to the intensity of wt controls (dotted red line equal to 1) introduced in the mutant or sh-RNA preparations (3 independent experiments, error bars are mean ± SD, two-tailed Student’s t-tests ∗p ≤ 5 × 10−2, ∗∗p ≤ 5 × 10−5, ∗∗∗p ≤ 5 × 10−8) wt n = 22 measurements from 22 germarium; mudf0 n = 24 measurements from 24 germarium; mud-RNAi (Bl:38190) n = 23 measurements from 23 germarium; mud-RNAi (Bl:35044) n = 23 measurements from 23 germarium.
Supplementary Figure 8
Projections of Z-sections obtained by confocal microscopy of fixed wild type (A) and mudf01205 (B) stage 3 egg chambers stained for C(3)G in red, the nuclear membrane (lectin, green), and DNA. When PCs are observed in mudf01205 the DNA in the corresponding oocyte is diffuse and lectin staining is absent.
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Dynamics of centromere clusters in region 1.
Time lapse microscopy (spinning disc) of a germarium expressing the centromere marker CID::RFP (red) and the fusome marker Par1::GFP (green). Three germinal stem cells (GSC) are identified by their position close to the niche and their spectrosome. The upper cystoblast (CB) is identified by its round fusome, and the 2-cell cyst (2cc), whose cells are linked by a snowman-shaped fusome. Four nuclei of an 8-cell cyst (8cc), whose cells are linked by a branched-shaped fusome, demonstrating that they are from the same cyst. Arrow points towards rotating centromeres cluster in an 8cc. Frames were taken every 10 s. The video is shown at 3 frames s−1 (MPEG4). (MP4 1083 kb)
Dynamics of Nuclear membrane in a rotating 8cc nucleus.
Time lapse microscopy (spinning disc) of a germarium expressing the centromere marker CID::RFP (red), the nuclear membrane marker Nup::GFP (green). Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 789 kb)
Dynamics of chromatin in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a germarium expressing the centromere marker CID::RFP (red) and the histone marker H2::dendra (green, red). Photo-conversion occurred just after the first z-acquisition, by applying 10 pulses of 0.054 s of 405 nm laser on the ROI. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 470 kb)
Centrosome and microtubules dynamics in living wild-type 8-cell cysts.
Time lapse microscopy (spinning disc) of a germarium expressing the centromere marker CID::RFP (red), the centrosome marker asl::YFP and the microtubule associated protein Jupiter::GFP (green). The movie is shown at 7 frames s−1 (MPEG4). (MP4 1013 kb)
Microtubule dynamics in UV pulse and Colcemid treated living 8-cell cysts.
Time lapse microscopy (spinning disc) of a colcemid-treated germarium expressing the centromere marker CID::RFP (red) and the microtubule-associated protein jupiter::GFP (green). A 5 s UV pulse was performed at t = 10: 00, illustrated by a light blue flash. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 1333 kb)
Microtubule, centrosomes and centromeres dynamics in UV pulse and Colcemid treated living 8-cell cysts.
Time lapse microscopy (spinning disc) of a colcemid-treated germarium expressing the centromere marker CID::RFP (red), the microtubule-associated protein jupiter::GFP (green) and the centrosome associated protein asterless::YFP (green). A 5 s UV pulse was performed at t = 2: 00, illustrated by a light blue flash. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). Filled arrowheads point to the fusome, empty arrowheads point to centrosome, and arrows point to the cell membrane (MPEG4). (MP4 370 kb)
Centrosomes rotate in the same direction and with the same speed as centromeres in living 8-cell cysts.
Time lapse microscopy (spinning disc) of germarium expressing the centromere marker CID::RFP (red) and the centrosome marker asl::YFP (green). Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 134 kb)
Colcemid treatment leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a colcemid-treated germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 251 kb)
Centromere dynamics in UV pulse and Colcemid treated in living 8-cell cysts.
Upper panel: Time lapse microscopy (spinning disc) of a colcemid-treated germarium expressing the centromere marker CID::RFP. A 5 s UV pulse was performed at t = 10: 00, illustrated by a light blue flash. Bottom panel: Tracking of two CID::RFP clusters before and after the UV pulse. The circles illustrates the maximal area covered before (yellow) and after (pink) UV pulse. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 528 kb)
Centrosome dynamics in UV pulse and Colcemid treated in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a living colcemid-treated germarium expressing the centromere marker CID::RFP (red), the centrosome marker asl::YFP and the microtubule associated protein Jupiter::GFP (green). A 5 s UV pulse was performed at t = 2: 00, illustrated by a light blue flash. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 445 kb)
Centromere dynamics in UV pulse and Colcemid treated in living stem cell.
Upper panel: Time lapse microscopy (spinning disc) of a colcemid-treated germarium expressing the centromere marker CID::RFP. A 5 s UV pulse was performed at t = 10: 00, illustrated by a light blue flash. Bottom panel: Tracking of two CID::RFP clusters before and after the UV pulse. The circles illustrates the maximal area covered before (yellow) and after (pink) UV pulse. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 622 kb)
white loss of function by RNAi does not affect CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a w-shRNA35573 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 399 kb)
sas-4 loss of function by shRNA leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a sas-4-shRNA35049 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 451 kb)
asl loss of function by shRNA leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a asl-shRNA35039 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 285 kb)
Dynein loss of function by shRNA leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a Dhc64C-shRNA36583 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 204 kb)
Dynein loss of function in Dhc64C3−2/Dhc64C6−12 mutant leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a Dhc64C3−2/Dhc64C6−12 mutant germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 168 kb)
Centrosome and microtubule dynamics in living Dynein mutant 8-cell cysts.
Time lapse microscopy (spinning disc) of a Dhc64c6−12/Dhc64c3−2 mutant germarium expressing the centromere marker CID::RFP (red), the centrosome marker asl::YFP and the microtubule associated protein Jupiter::GFP (green). The movie is shown at 7 frames s−1 (MPEG4). (MP4 1018 kb)
CID-RFP and KASH-GFP remain in close proximity in living 8-cell cysts.
Time lapse microscopy (spinning disc) of germarium expressing the centromere marker CID::RFP (red) and the KASH domain KASH::GFP (green). Frames were taken every 20 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 201 kb)
klarsicht loss of function leads to inhibition of CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a klarmarbCD4 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 219 kb)
klaroid loss of function displays CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a koi80 germarium expressing the centromere marker CID::RFP. Frames were taken every 10 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 363 kb)
CID foci dynamics in wild type 8-cell cysts.
Time lapse microscopy (spinning disc) of a germarium expressing the centromere marker CID::RFP. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 121 kb)
mud loss of function does not affect CID foci dynamics in living 8-cell cysts.
Time lapse microscopy (spinning disc) of a mudf01205 mutant germarium expressing the centromere marker CID::RFP. Frames were taken every 30 s. The movie is shown at 7 frames s−1 (MPEG4). (MP4 11 kb)
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Christophorou, N., Rubin, T., Bonnet, I. et al. Microtubule-driven nuclear rotations promote meiotic chromosome dynamics. Nat Cell Biol 17, 1388–1400 (2015). https://doi.org/10.1038/ncb3249
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DOI: https://doi.org/10.1038/ncb3249
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