Histone H3K9 and H4 Acetylations and Transcription Facilitate the Initial CENP-AHCP−3 Deposition and De Novo Centromere Establishment in Caenorhabditis elegans Artificial Chromosomes
The centromere is the specialized chromatin region that directs chromosome segregation. The kinetochore assembles on the centromere, attaching chromosomes to microtubules in mitosis. The centromere position is usually maintained through cell cycles and generations. However, new centromeres, known as neocentromeres, can occasionally form on ectopic regions when the original centromere is inactivated or lost due to chromosomal rearrangements. Centromere repositioning can occur during evolution. Moreover, de novo centromeres can form on exogenously transformed DNA in human cells at a low frequency, which then segregates faithfully as human artificial chromosomes (HACs). How centromeres are maintained, inactivated and activated is unclear. A conserved histone H3 variant, CENP-A, epigenetically marks functional centromeres, interspersing with H3. Several histone modifications enriched at centromeres are required for centromere function, but their role in new centromere formation is less clear. Studying the mechanism of new centromere formation has been challenging because these events are difficult to detect immediately, requiring weeks for HAC selection.
DNA injected into the Caenorhabditis elegans gonad can concatemerize to form artificial chromosomes (ACs) in embryos, which first undergo passive inheritance, but soon autonomously segregate within a few cell cycles, more rapidly and frequently than HACs. Using this in vivo model, we injected LacO repeats DNA, visualized ACs by expressing GFP::LacI, and monitored equal AC segregation in real time, which represents functional centromere formation. Histone H3K9 and H4 acetylations are enriched on new ACs when compared to endogenous chromosomes. By fusing histone deacetylase HDA-1 to GFP::LacI, we tethered HDA-1 to ACs specifically, reducing AC histone acetylations, reducing AC equal segregation frequency, and reducing initial kinetochroe protein CENP-AHCP−3 and NDC-80 deposition, indicating that histone acetylations facilitate efficient centromere establishment. Similarly, inhibition of RNA polymerase II-mediated transcription also delays initial CENP-AHCP-3 loading.
Acetylated histones on chromatin and transcription can create an open chromatin environment, enhancing nucleosome disassembly and assembly, and potentially contribute to centromere establishment. Alternatively, acetylation of soluble H4 may stimulate the initial deposition of CENP-AHCP−3-H4 nucleosomes. Our findings shed light on the mechanism of de novo centromere activation.
KeywordsDe novo centromeres Neocentromeres Centromere establishment Artificial chromosomes Epigenetics Chromatin environment Histone modifications Histone acetylations
The centromere is a chromatin region specialized for chromosomes segregation. Its function is to attach the chromosome through the kinetochore complex to the microtubule spindle fibers, which pull sister chromatids apart during anaphase in mitosis. Centromeric regions have different DNA sequences and sizes across species, but functional centromeres are often marked by the conserved histone H3 variant, CENP-A. Neocentromeres occasionally form on ectopic regions after chromosomal rearrangements or inactivation of the original centromere . Centromere repositioning also occurs during speciation despite gene synteny maintenance . Moreover, de novo centromeres can form on exogenous DNA transformed into cells, which then segregates faithfully as artificial chromosomes (ACs). These functional neocentromeres and de novo centromeres also contain CENP-A. Thus, CENP-A is believed to be the primary epigenetic mark to maintain centromere identity. CENP-A is also recognized as one of the most upstream proteins in the kinetochore assembly hierarchy and acts as a platform to recruit other kinetochore proteins [3, 4].
Interestingly, CENP-A nucleosomes replaces some canonical H3 nucleosomes in the centrochromatin region , but CENP-A nucleosomes do not occupy all centrochromatin in regional monocentromeres and holocentromeres studied. Instead, they intersperse with H3 nucleosomes [6, 7]. Specific histone modifications on H3 and CENP-A nucleosomes are enriched at centromeres, and some are important for centromere function. For example, histone H3 lysine 4 dimethylation (H3K4me2), which is associated with active transcription, is enriched at human and Drosophila centromeres by chromatin fiber analysis, while H3 and H4 acetylations and heterochromatin marks, H3K9me2/3, are under-represented in the centrochromatin region [8, 9, 10]. This shows that the centrochromatin resembles neither typical euchromatin nor heterochromatin. H3 and H4 hypoacetylations are important for centromere function in S. pombe . On the contrary, an enrichment of H3K9me3 and a low level of H3K4me2 are found in centromeres of chicken DT40 cells . H4K20me1, which is associated with transcriptional activation , is highly enriched in human and chicken CENP-A nucleosomes, and is required for kinetochore function . H3T3ph, which is associated with mitosis, is also found in human and chicken centromeres and is responsible for the localization of Aurora B [12, 15, 16]. H2B monoubiquitination (H2Bub1), which is involved in replication, transcription and DNA repair, is found in human and S. pombe centromeres and is important for proper chromosome segregation in S. pombe and S. cerevisiae [17, 18, 19, 20, 21, 22]. In holocentric C. elegans, H3K27me3 and H3K9me3 positively correlate with CENP-A domains [7, 23, 24], but a reduction in H3K27me3 did not affect CENP-A localization . In addition, several CENP-A modifications have been shown to be important for centromere function, including human CENP-A glycine 1 (G1) trimethylation, which aids the interaction with alpha-satellite DNA; S16 and 18 phosphorylation, which compacts the CENP-A nucleosomal array ; and K124 ubiquitination, which is required not only for the maintenance of the old CENP-A, but also for the recruitment of the newly synthesized CENP-A . However, whether these histone modifications only regulate existing centromere maintenance, or also affect centromere activation and inactivation are not clear.
The processes of centromere activation and inactivation, despite important for chromosome stability, are not easy to capture and study due to their infrequent occurrences. For instance, human ACs (HACs) form at a low frequency (0–30%) after the introduction of naked alpha-satellite repetitive DNA and require 6 weeks of selection . Recently, the development of HACs carrying a synthetic, higher-order alpha-satellite repeat array with tet operator (tetO) sequence inserted in every other alphoid monomer has facilitated the modulation of the de novo centromere chromatin environment on HACs by targeting the tet repressor (tetR) fused with a specific histone modifier or transcriptional regulator [29, 30]. The effects of several histone modifications have been studied on stably maintained de novo centromeres on HACs, which have already propagated through multiple cell cycles. These stably maintained de novo centromeres, as in natural centromeres, contain pre-existing CENP-A nucleosomes to build the kinetochore in mitosis and mark the centromere identity for propagation through cell cycles and generations. H3K4me2 was shown to be required for CENP-A chaperone HJURP targeting and CENP-A assembly on stably maintained de novo centromeres on HACs . However, tethering of either a transcriptional activator or repressor induces different degrees of HAC loss, suggesting that a balance between open and closed chromatin and transcriptional level may be required for the maintenance of de novo centromeres [29, 30]. The propagating mechanisms of de novo centromeres potentially resemble those of endogenous centromeres.
On the other hand, during the de novo centromere formation and stabilization process, new CENP-A nucleosomes are first incorporated at an ectopic site and subsequently propagated at this specific location. New centromere establishment may require different or additional histone modifications when compared with centromere propagation. However, the role of histone modifications in de novo centromere formation or maturation is not well understood. A previous study in HACs showed that H3K9ac and H3K9me3 promotes and inhibits HAC formation, respectively . Despite the recent advances in HAC construction methods , generation of a large number of HACs to directly observe de novo centromere formation events remains difficult due to the low HAC formation rate and long selection time. In addition, HACs could only be formed in a limited number of human cell lines, possibly due to the differences in the chromatin environment [28, 32]. This may limit the use of HACs as de novo centromere models and their applications as cloning vectors.
In order to study the process of de novo centromere formation more directly, an in vivo system for rapidly generating visualizable new ACs in Caenorhabditis elegans has been developed . In C. elegans, DNA injected into the gonad can concatemerize to form ACs, also known as extrachromosomal arrays (Ex), in embryos produced from the injected gonad [35, 36]. These ACs are commonly used to express transgenes in worms. Yet, even non-C. elegans DNA sequences are capable of forming ACs, possibly because the regulation of centromeres depends heavily on epigenetics and not on DNA sequences in holocentromeres . By live-cell imaging, these newly formed, first-generation ACs first undergo passive inheritance, but soon gain autonomous segregation ability within a few cell cycles . By immunofluorescence, inner and outer kinetochore proteins assemble on ACs that have been propagated for a few generations, indicating the establishment of de novo centromeres . Interestingly, these ACs do not hitch-hike on endogenous chromosomes, but congress and align independently onto the metaphase plate . Importantly, C. elegans ACs gain de novo centromeres more rapidly (by 64-cell stage, after 6 cell divisions, within 200 min of fertilization)  and at a higher frequency than HACs. Previously, we showed that inhibition of the heterochromatin protein HP1 increases the segregation frequency in 1-cell stage, suggesting heterochromatin may hinder de novo centromere formation . Here, we utilize this system to study the role of histone modifications and transcription in C. elegans ACs. We show that newly formed C. elegans ACs are hyperacetylated at H3K9 and H4K5/8/12/16 compared to endogenous chromosomes, and this hyperacetylation and associated transcription promote efficient de novo centromere formation on C. elegans ACs. Our work demonstrates the use of C. elegans ACs as an in vivo model to study the role of epigenetic factors in de novo centromere formation during the actual time of the event, and illustrates the involvement of histone acetylation and transcription in de novo centromere establishment.
Caenorhabditis elegans newly formed ACs in early cell stage are hyperacetylated at H3K9 and H4
In heritable ACs that have been propagated for multiple generations, the acetylation levels are very low (and they do not vary at different cell stages) (Fig. 1c, d and Additional file 2: Fig. S2). This result is consistent with the findings that repetitive propagated ACs are enriched with H3K9me3 (Additional file 4: Fig. S4) . Interestingly, the reduction in acetylation levels on propagated ACs in GFP::LacI::HDA-1-tethering strain is more severe than that in GFP::LacI-tethering strain (Fig. 1c, d), possibly due to the deacetylase activity of the HDA-1.
Reducing H3K9ac/H4ac on newly formed ACs in C. elegans delays their ability to achieve accurate segregation
To investigate whether the histone acetylation on ACs plays a role in de novo centromere formation, we tethered HDA-1, a histone deacetylase expressed in C. elegans embryos [39, 40, 41], specifically to LacO-containing ACs by constructing a strain expressing GFP::LacI::HDA-1 under hda-1 endogenous promoter (Additional file 8: Table 1). To verify the function of GFP::LacI::HDA-1 on ACs and confirm that it does not affect histone acetylation on endogenous chromosomes, immunofluorescence was performed to detect H3K9ac and H4ac levels in the GFP::LacI::HDA-1-tethering strain, and compared to those in the GFP::LacI-tethering strain and the enzymatically dead GFP::LacI::HDA-1(H145A)-tethering strain, in which HDA-1 has a point mutation at the deacetylase domain . Both H3K9ac and H4ac levels on newly formed LacO ACs in 1 to 32-cell stage on GFP::LacI::HDA-1-tethering strain are significantly lower than those on GFP::LacI-tethering strain (Fig. 1c and d). On the other hand, H3K9ac and H4ac levels on new ACs tethered with GFP::LacI::HDA-1(H145A) are comparable to those tethered with GFP::LacI alone (Additional file 5: Fig. S5). This shows that the effect on ACs is specific to the deacetylase enzymatic activity of HDA-1 and not just due to the bulky tethering. Moreover, both H3K9ac and H4ac levels on endogenous chromosomes of GFP::LacI::HDA-1-tethering embryos have not decreased significantly, when compared to endogenous chromosomes of GFP::LacI-tethering embryos (Fig. 1c, d), indicating that GFP::LacI::HDA-1 are able to target LacO ACs specifically to decrease proximal histone acetylations without significantly affecting histone acetylation level on endogenous chromosomes.
Histone H3K9 and H4 acetylations facilitate the initial CENP-AHCP−3 and NDC-80 deposition on the de novo centromere on newly formed ACs
Interestingly, the amount of CENP-AHCP−3 and NDC-80 signals on newly formed ACs increased with embryonic divisions (Fig. 3a, c), consistent with the rise in segregation frequency over time (Fig. 2), suggesting that the de novo kinetochore becomes more mature and functional over time. Indeed, the average signal intensity of CENP-AHCP−3 and NDC-80 on 17 to 32-cell stage first-generation ACs in GFP::LacI-tethering strains becomes comparable to those on propagated ACs and endogenous chromosomes, which segregate equally (Fig. 3a). The difference in segregation frequency and CENP-AHCP−3 between these two strains can only be observed in first-generation ACs at early embryo stage. In consistence with the signal increase of CENP-AHCP−3 on the newly formed ACs over time, CENP-AHCP−3 orientation changes from diffuse (100% in 1 to 8-cell stage) to bi-oriented (45% in 17 to 32-cell stage) in GFP::LacI-tethering strain (Fig. 3b). The mechanism behind this natural maturation of centromere in GFP::LacI-tethering strain is not completely clear.
Histone acetylations are correlated with active transcription on newly formed ACs during centromere formation, but transcription is not required for maintenance of centromere
In this study, we investigated the relationship between histone modifications, transcription and de novo centromere establishment. We suggest that in order for a de novo centromere to efficiently form and function, two categories of epigenetic mark or histone modifications may be required. The first ones are seeding marks that favor incorporation of CENP-A nucleosomes or other centromeric proteins into ectopic, originally non-centromeric regions. Such marks may help to establish a de novo centromere identity. Once established, the second group of epigenetic marks may reinforce the centromere identity and propagates the de novo centromere through mitosis and meiosis, such as histone modifications that help with centromere licensing and new CENP-A deposition during every cell cycle. The histone modifications that propagate endogenous existing centromeres and stably maintained de novo centromeres appear to be the same [29, 30]. However, histone modifications affecting de novo centromere establishment are less clear. A previous study in HACs has found that euchromatin mark H3K9ac promotes de novo centromere formation, whereas the heterochromatin mark H3K9me3 antagonizes de novo centromere formation . Interestingly, once the de novo centromere is established, H3K9ac is no longer needed .
To seed a new centromere, CENP-A or other epigenetic marks of the centromere must be ectopically incorporated into non-existing centromeric chromatin. No matter whether these epigenetic marks are deposited by a chaperone, histone modifier or incorporated autonomously, an open chromatin will be more accessible to these proteins. We hypothesized that an open chromatin may be advantageous for new CENP-A incorporation in a replication-independent manner. Although both H3/4 acetylations and H3K4me2 are open chromatin marks associated with active transcription [47, 48], they may influence chromatin structure through different mechanisms. H3K4me2 allows binding of specific transcription factors or chromatin remodelers to influence transcription [49, 50, 51]. H3/4 acetylations open the chromatin structure by adding an acetyl group to lysine to remove its positive charge, thereby loosening the interaction between histones and the wrapping DNA, and resulting in increased histone turnover [52, 53, 54, 55]. Moreover, H3/4 acetylations have the ability to recruit specific proteins, such as bromodomain-containing proteins, as histone readers to the modified chromatin [56, 57, 58], and allow transcription factors and RNA polymerase to bind to mediate transcription. H3/4 acetylations also have broader chromatin functions, such as in DNA replication and DNA damage repair [59, 60]. Thus, open chromatin marks such as H3/4 acetylations may contribute to efficient de novo centromere formation by facilitating nucleosome disassembly and assembly, and initial CENP-A incorporation (Fig. 3). Alternatively, acetylation on newly synthesized histones, such as H4K5/12ac, may affect the nuclear transport and deposition of soluble CENP-A-H4 tetramers . Based on this hypothesis, a previous HAC study has shown the role of H3K9 acetylation using a HAC formation assay by a 6-week selection process followed by fluorescence in situ hybridization (FISH)-immunofluorescence analysis . In consistence, we detected hyperacetylations on H3K9 and H4 in early (1 to 8-cell stage), first-generation LacO-containing ACs formed in C. elegans embryos (Fig. 1c, d). We further showed that H3/4 hyperacetylations on ACs contribute to its rapid segregation capability (Fig. 2) and de novo centromere formation (Fig. 3) in a whole organism model.
Although H3/4 acetylations contribute to de novo centromere formation based on our study and the HAC study , whether they function in centromere maintenance is less clear. Previous studies have shown that H3/4 hypoacetylation occur in human and Drosophila endogenous centromeric region , as well as in S. pombe centromeric inner and outer repeats [62, 63, 64]. The heterochromatin and histone hypoacetylation flanking the regional centromere, such as those present in S. pombe outer repeats, are thought to recruit cohesin to keep sister chromatids together . In C. elegans, the heterochromatin is at the arms of the chromosomes but not exactly flanking the holocentromeres, so the role of heterochromatin and hypoacetylation in holocentromere function or cohesion remains unclear. Recently, endogenous human centromeres are shown to be acetylated temporarily before new CENP-A is deposited [32, 64]. Tethering of a histone acetyltransferase even partially rescued the CENP-A assembly defect on established HACs in hMis18α depletion [32, 54]. In C. elegans, RbAp46/48LIN−53, known to associate with HAT-1TAG−235 , is required for CENP-A assembly on endogenous holocentric chromosomes, but HAT-1TAG−235 depletion does not affect endogenous chromosome segregation . In contrast to de novo centromeres, existing, endogenous centromeres do not require ectopic CENP-A or other centromeric proteins to be incorporated into non-centromeric chromatin. Open chromatin marks that are advantageous for the initial deposition of centromeric proteins onto de novo centromeres on ACs may not be required for stably maintained centromeres (Fig. 6b). Other mechanisms, including the involvement of CENP-A chaperones, may be sufficient to propagate the existing centromeres.
Transcription is associated with nucleosome remodeling and chromatin modification processes. For instance, some transcriptional adaptor proteins containing the acetyltransferase subunit can acetylate histone H3 and H4 at specific lysines by to make the chromatin more accessible for gene activation [67, 68]. Alternatively, acetylation of soluble H4 may stimulate the initial deposition of CENP-AHCP−3-H4 nucleosomes . In humans, centromeres are transcribed during G1 phase , coinciding with the time of CENP-A deposition. Centromeric transcription may couple with nucleosome exchange to incorporate CENP-A nucleosomes into centromeric, open chromatin [70, 71, 72]. In C. elegans, gene transcription has been shown to begin at 4-cell stage . We detected transcription initiation on newly formed GFP::LacI-tethered ACs, especially at early embryo stages (Fig. 4). Inhibition of RNA Pol II reduces the level of CENP-A on newly formed ACs (Fig. 5b), and ACs equal segregation frequency (Fig. 5c). Histone deacetylation of newly formed ACs reduces transcription initiation on ACs, especially at 1 to 8-cell stage (Fig. 4), and reciprocally, inhibition of RNA Pol II reduces H3K9 and H4 acetylation on ACs (Additional file 7: Fig. S7), confirming the interdependent relationship between histone acetylation and transcription. These results suggest that transcription, together with histone acetylation, can epigenetically regulate de novo CENP-AHCP−3 loading and centromere formation. Surprisingly, CENP-AHCP−3 domains are indeed negatively correlated with RNA Pol II (r = − 0.66), H3K36me2/3 (r = − 0.6) and H3K4me2 (r = − 0.49) occupancy on endogenous C. elegans chromosomes [7, 23]. Moreover, transcription does not affect CENP-AHCP−3 maintenance on repetitive propagated ACs (Fig. 5b) and on endogenous chromosomes in C. elegans . Such difference in the effect of transcription may be attributed to the mechanism of de novo centromere formation and centromere propagation of existing centromeres.
In human cells, HAC formation (up to 30% in HT1080 cell line) is identified after 6 weeks of selection, transformant isolation and confirmation of the presence of CENP-A on HACs without genomic integration [31, 32]. In C. elegans, an average of 3 ACs was observed in 1-cell stage embryos without further increase in later cell stage , suggesting that AC formation finishes by 1-cell stage, and enabling the tracing of a large population of individual ACs for analysis. By 64-cell stages (in 6 cell divisions, < 200 min since fertilization) , the majority of mitotic cells containing ACs (84%) contain ACs that can equally segregate. This provides an efficient model for de novo centromere formation. Moreover, any DNA sequence can be injected for AC formation in C. elegans [6, 7, 24, 34, 74], but alpha satellites must be transfected for HAC formation in human cells. The difference in de novo centromere formation rate in C. elegans and humans may be related to the plasticity nature of holocentromeres in C. elegans. The kinetochore protein complexes on holocentromeres are largely similar to those on monocentromeres [6, 34, 74]. No centromere-specific sequences have been identified in C. elegans, although GA-rich motifs, which coincide with transcription factor high occupancy target (HOT) sites, are common to the centromeric sites . Besides, CENP-AHCP−3 domains are positively correlated with H3K27me3 (r = 0.64) and H3K9me3 (r = 0.44) [7, 23, 24]. These findings suggest that holocentromere regulation is largely epigenetic. Therefore, de novo centromere formation in holocentromeres may be more promiscuous than in monocentromeres.
Our study applied a straightforward functional assay to monitor de novo centromere formation. In addition to measuring the final stable AC formation rate as in HAC studies, we can also observe the change in AC segregation frequency in different embryo stages. By live-cell imaging of consecutive cell divisions in early embryos of C. elegans, we can directly observed a first-generation AC matures from undergoing passive inheritance in one division to equally segregating in the next mitosis, implicating a de novo centromere formation event . Using this real-time method, we were able to pinpoint the formation time of each de novo centromere down to a particular cell cycle, and track the fate of the AC in subsequent divisions. Currently, how and why ACs matures over time naturally is still not fully understood. Albeit tethering of HDA-1 histone deacetylase or inhibiting transcription can delay the formation of de novo centromeres on ACs, they eventually can be matured and stably propagated (Fig. 6a). How CENP-AHCP−3 initially loads and form de novo centromere even in H3K9/H4 hypoacetylated environment remains an open question. The real-time observation approach without selection offers a valuable opportunity to better understand the mechanism underlying de novo centromere establishment in vivo. We can temporally monitor histone modifications, kinetochore protein levels and chromosome segregation at different embryo cell stages, from before the establishment of a functional centromere to after. In this study, we use a protein tethering approach based on LacO:LacI binding to specifically recruit a histone modifier to ACs, analogous to previous studies in HACs, where tetO sequences were inserted to centromeric alpha-satellite DNA [28, 29, 30, 31, 32, 33]. In contrast to the application of a drug against a histone modifier, which affects the whole cell with pleiotropic effects, our genetic engineering method is intended not to affect the endogenous chromosome chromatin environment and thus is more specific.
Our study also demonstrates a direct way to manipulate the AC chromatin environment in order to study de novo centromere formation, which may help to design ACs that segregate more faithfully, a crucial factor for their use as cloning vectors. The size of the GFP foci binding to the ACs does not change through the embryo stages since 1-cell stage , suggesting the size of the ACs does not increase over time. However, one of the caveats in our cytological assay is that we were not able to isolate these newly formed, first-generation ACs for biochemical analyses, including chromatin immunoprecipitation (chIP) to investigate DNA–protein interactions. On the other hand, we could isolate stable, propagating ACs for chIP study. Live imaging and chIP analyses of ACs should complement each other to obtain high temporal resolution of centromere establishment dynamics, and high sequence resolution of de novo centromere architecture, respectively.
Here, we showed that histone acetylations facilitate efficient de novo centromere formation. Moreover, our study implicated that the histone acetylation and transcription-driven de novo centromere establishment is not just an aberrant event that merely occurs in cancer cells or cell lines; rather, it can also occur in physiologically normal cells in whole organisms and thus is biologically relevant. Likely, a balance between de novo centromere formation and suppression is necessary for maintaining genome stability in development and evolution.
Worm strain construction and DNA injection
All strains were maintained at 20 °C. WYY7 (unc-119(ed3)III; hkuSi2[hda-1p::GFP::LacI::hda-1; cb-unc-119(+)(WYYp33)]II; ltIs37 [pie-1p::mCherry::his-58 (pAA64) + unc-119(+)]) was made by inserting a single copy of GFP::LacI::HDA-1 (genomic DNA with introns) into EG6699 using MosSCI [75, 76] and subsequently crossed with OD56 to obtain a double homozygous of GFP::LacI::HDA-1 and mCherry::H2B (Additional file 8: Table 1). The GFP::LacI::HDA-1 is regulated by 2.5 kb of endogenous hda-1 promoter and a 0.6 kb of hda-1 3′ UTR sequence. WYY28 (unc-119(ed3)III; hkuSi6[Phda-1:: GFP::LacI::hda-1(H145A)::hda-1 3′UTR; cb-unc-119(+)(WYYp112)]II; ltIs37 [pie-1p::mCherry::his-58 (pAA64) + unc-119(+)]) was made by PCR site-directed mutagenesis of WYYp33 to mutate histidine at residue 145 to alanine (H145A), and constructed similarly to WYY7 (Additional file 8: Table 1). A mixture of purified p64xLacO plasmid (100 ng/μl) and pRF4 plasmid (50 ng/μl), carrying the rol-6(su1006) dominant marker, which gives a roller phenotype in larva and adults, was co-injected into gonad of young adult worms with standard procedure . Worms were recovered at 20 °C for 4–8 h before subsequent live imaging or immunofluorescence of newly formed ACs. Propagated ACs were constructed by selecting F1 and next-generation worms that roll.
Worms were dissected on polylysine-coated glass slides in a droplet of M9 buffer. Samples were then flattened with a glass cover slip and freeze-cracked in liquid nitrogen. Samples were fixed in cold methanol for 30 min. They were stained with primary antibodies (0.93 mg/ml mouse monoclonal anti-LacI (Millipore 05-503), 1.16 mg/ml rabbit polyclonal anti-H3K4me2 (Novus Biologicals NB21-1022), 1 mg/ml rabbit polyclonal anti-H3K9ac (Millipore ABE18), 1 mg/ml rabbit polyclonal anti-H4ac, which recognizes H4K5ac, H4K8ac, H4K12ac and H4K16ac (Millipore 06-598), 1 mg/ml rabbit polyclonal anti-Histone H3 (Abcam ab1791), 1 mg/ml rabbit polyclonal anti-Histone H4 (Abcam ab10158), 1 mg/ml rabbit polyclonal anti-CENP-AHCP−3 (Novus Biologicals 29540002), 1 mg/ml rabbit polyclonal anti-NDC-80 (OD32, a gift from Arshad Desai) and 0.8 mg/ml rabbit polyclonal anti-RNA Polymerase II phospho Ser5 (Ser5P) (Abcam ab5131)) diluted 1:500 (or 1:1000 for CENP-AHCP−3 and NDC-80 antibodies) in Abdil buffer and then stained with 0.75 mg/ml fluorescence-conjugated secondary antibodies [anti-Rabbit IgG-Alexa 647 (Jackson Immuno Research 111-606-045) and anti-Mouse IgG-FITC (Jackson Immuno Research 115-096-062)] diluted 1:500 in PBST as previously described . IF slides were imaged with a Carl Zeiss LSM780 laser scanning confocal microscope with a Plan-Apochromat 40× Oil objective and PMT detectors. Stacks with 25 × 0.5 μm planes were scanned for each embryo in a 4× zoom. DAPI, FITC and Alex647 channels were scanned with a 2.55 μs pixel dwell time and 36 μm pinhole for all 3 channels. The images were saved in 16 bits format. At least 2 independent experiments have been performed, using the same batch of antibody solution.
Immunofluorescence signal quantification
To define the areas of measurement for each individual AC or the bulk endogenous chromosomes, a region of interest (IROI) enclosing the AC (based on LacI) or endogenous chromosomes was selected and a slightly larger region enclosing the ROI (LROI) was drawn. The total LacI, histone modification, CENP-AHCP−3, NDC-80, RNA Pol II Ser5P or DAPI signal intensity was measured in the ROI (IROI) and LROI (ILROI) for each AC and endogenous chromosomes. The mean background signal intensity (ib) was calculated by subtracting the total intensity in ROI from the total intensity in LROI and then divided by the area in between the two ROIs (ALROI − AROI) (i.e. ib = (ILROI − IROI)/(ALROI − AROI)). The background signal intensity in ROI (BROI) was calculated by multiplying the mean background signal intensity by the area in ROI (i.e. BROI = ib × AROI). The total corrected signal in ROI (CROI) was calculated by subtracting the background signal in ROI from the signal in ROI (CROI = IROI − BROI). The mean corrected signal (cROI) was calculated by the total corrected signal in ROI divided by the area in ROI (i.e. cROI = CROI/AROI). Then, the mean-corrected LacI, histone modification, CENP-AHCP−3, NDC-80 or RNA Pol II Ser5P signal was normalized with the mean-corrected DAPI signal in the same ROI (e.g. normalized mean corrected LacI signal NROI LacI = cROI LacI/cROI DAPI).
Worms were dissected in M9 buffer droplets to release embryos. Embryos were mounted on agarose pads for imaging. Live images were taken with a Carl Zeiss LSM710 laser scanning confocal microscope with an EC Plan-Neofluar 40× Oil objective and PMT detectors. Stacks with 12 to 14 × 1.8 μm planes were scanned for each embryo in a 3.8× zoom and a 2-min or 30-s interval, or stacks with 25 × 0.6 μm planes were scanned for each embryo in a 1.6× zoom. Red and green channels were scanned simultaneously with a 2.55–6.3 μs pixel dwell time and 31–62 μm pinhole. The images were saved in 16 bits format.
AC segregation scoring was performed as described previously . Every dividing cell that contains at least one AC was counted as one sample. Each division was categorized as either containing at least a segregating AC or containing (all) non-segregating AC(s). Segregating ACs were defined as those that aligned with the metaphase plate and segregated equally with endogenous chromosomes during anaphase. Non-segregating ACs include those that did not align with the metaphase plate, or missegregated during anaphase. The segregation rate was then calculated as the number of dividing cells containing segregating ACs over the total number of dividing cells containing ACs.
Embryo permeabilization and drug treatment
To obtain permeabilized C. elegans embryos, the T01H3.4 clone from the Ahringer library  was used for perm-1 RNAi by feeding. Bacteria expressing dsRNA targeting perm-1 were grown overnight at 37 °C in LB with 100 mg/ml ampicillin. The overnight culture was diluted 1:50 in LB with 100 mg/ml ampicillin and grown at 37 °C until the culture reached an OD600 around 0.4 (2.5–3 h). The bacterial culture (200 ml/plate) was spread onto NGM agar plates containing 0.01 mM IPTG. Plates were dried in a sterile hood for 1 h and left at room temperature for 4 additional hours to induce the RNA expression . Around 30 L4 stage worms were then transferred onto the plate and incubated overnight at 20 °C for 12–14 h. Then, a mixture of purified p64xLacO plasmid (100 ng/μl) and pRF4 plasmid (50 ng/μl) was co-injected into the gonad of adult worms as described. Worms were recovered at 20 °C for 6 to 8 h on another perm-1 feeding RNAi plate before subsequent immunofluorescence or live imaging of newly formed ACs. For immunofluorescence, α-amanitin (Abcam ab144512) was diluted to the working concentration (200 μg/ml) in 0.7× Egg salt buffer (1× Egg salt buffer: 118 mM NaCl, 40 mM KCl, 3.4 mM MgCl2, 3.4 mM CaCl2, 5 mM HEPES pH 7.4). Embryos were dissected in 200 μg/ml α-amanitin and incubated for 30 min before performing immunofluorescence. 2 μl Latex beads (15 μm, 74964 Sigma-Aldrich) were added to protect the permeabilized embryos from damage by the coverslip. Immunofluorescence was performed as described above. For live imaging, the microdevice well was filled with 80 μl 0.7× Egg salt buffer . Worms were dissected on the dissection board, and the embryos were swept to the wells by an eyelash tool. The medium in the well was exchanged by removing the existing medium using a syringe and adding fresh medium with 200 μg/ml α-amanitin with a pipette, and incubated for 30 min. Then, live imaging of the embryos was performed as described above.
JZ, KCLC and KWYY were involved in conceptualization; JZ, KCLC and KWYY contributed to methodology; JZ, KCLC and KWYY were involved in investigation; JZ and KCLC were involved in formal analysis; KCLC and KWYY wrote the original draft; JZ and KWYY contributed to writing—review and editing; JZ, KCLC and KWYY was involved in Visualization; KWYY acquired funding; KWYY contributed to resources, supervision, and project adminstration. All authors read and approved the final manuscript.
We thank Arshad Desai for critical reading of the manuscript and comments. We thank Rachel Chan and Abby Mak for technical assistance. We are grateful to the University of Hong Kong School of Biological Sciences Central Facilities and Li Ka Shing Faculty of Medicine Faculty Core Facility for the microscopy facility.
The authors declare that they have no competing interests.
Availability of data and materials
The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request.
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This project is supported by the HK Research Grant Council (RGC) Early Career Scheme (ECS) Award (Project No. 788012) and the HKU Seed Fund for Basic Research (Project No. 201411159195).
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