2 Department of Pathology, Biochemistry, and Cancer Biology, Medical College of Ohio, Toledo, OH 43614
3 Department of Radiation Oncology, New England Medical Center, Tufts University School of Medicine, Boston, MA 02111
Correspondence to Qingshen Gao: q-gao{at}northwestern.edu
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Abbreviations used in this paper: cDNA, complementary DNA; HU, hydroxy urea; RNAi, RNA interference; siRNA, small interfering RNA.
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Introduction |
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In mammalian cells, the centrioles consist of nine triplets of microtubules, arranged in a cylinder that has a 200-nm diameter and an 500-nm length, with additional filaments, fibers, and dense material attached to or inside of the microtubular cylinder (Doxsey, 2001; Beisson and Wright, 2003). In addition to
/ß-tubulin, only a small number of proteins have been found to localize to the centrioles in mammalian cells. These include centrin,
-tubulin, centriolin, ninein, and poly(ADP-ribose) polymerase-3 (Salisbury, 1995; Paoletti et al., 1996; Chang and Stearns, 2000; Mogensen et al., 2000; Piel et al., 2000; Ou et al., 2002; Augustin et al., 2003). The centrioles duplicate once per cell cycle in a manner similar to DNA replication. Centriole duplication starts at the onset of the S phase; the two centrioles separate and a new (daughter) centriole forms in association with the mother centriole (Rieder and Borisy, 1982; Vorobjev and Chentsov Yu, 1982). However, exactly how this protein-based structure duplicates accurately remains completely unknown. It has been clearly established that centrosome duplication in mammalian somatic cells requires CDK2 activity (Hinchcliffe et al., 1999; Lacey et al., 1999; Meraldi et al., 1999). Recently, nucleophosmin, Mps1p, and CP110 have been identified as centrosomal substrates of CDK2 and have also been shown to play an important role in the duplication of centrosomes (Okuda et al., 2000; Fisk and Winey, 2001; Chen et al., 2002).
The fidelity of mammalian cell division requires the precise segregation of genetic material into daughter cells, together with a well orchestrated distribution of subcellular organelles. Errors in this process are associated with genetic diseases and underlie aneuploidy, which is a hallmark of cancer progression. Normal centrosome duplication is a key requirement for the correct segregation of chromosomes during cell division, and the centrosome duplication cycle is tightly coupled to the cell division cycle (Doxsey, 2001; for review see Hinchcliffe and Sluder, 2001). Uncoupling of the centrosome duplication cycle from the cell division cycle leads to more than two centrosomes per cell, i.e., centrosome amplification, which is a phenotype frequently observed in both cultured tumor cells and a variety of human tumors (Lingle et al., 1998, 2002; Pihan et al., 1998, 2003; D'Assoro et al., 2002). Thus, the identification and characterization of novel centrosomal proteins that regulate centrosomal duplication is an area of cell biological and medical interest.
We have identified a novel daughter centrioleassociated protein that we have designated centrobin (centrosomal BRCA2 interacting protein). RNA interference (RNAi)mediated depletion of centrobin blocked centriole duplication and led to centrosomes with one or no centriole, demonstrating that centrobin is required for the assembly of the nascent centriole. Inhibition of centriole duplication upon centrobin depletion led to the impairment of cytokinesis. These studies identified a novel component of the daughter centriole that is essential for centriole duplication and function.
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Results |
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To examine the expression and function of centrobin, we generated an anti-centrobin antiserum against a His-tagged fusion protein of the COOH-terminal 539 aa of centrobin. To determine whether this antiserum specifically recognizes recombinant and endogenous centrobin, cell lysates from various cell lines and 293T cells transfected with vector, Myc-tagged centrobin, or GFP-tagged centrobin were analyzed by Western blotting using affinity-purified anti-centrobin antibody. Consistent with the size of centrobin, the anti-centrobin antibody recognized a 100-kD protein in all cell lines tested (Fig. 1 F, lanes 39). As expected, we found that the level of this 100-kD protein is significantly higher in the Myc-centrobintransfected 293T cells than in the vector-transfected cells (Fig. 1 F, lanes 3 and 4). Anti-Myc antibody specifically detected the 100-kD band only in the Myc-centrobintransfected cells (Fig. 1 F, lane 2). The specificity of the antiserum was also demonstrated by the presence of a 127-kD protein in the GFP-centrobintransfected 293T cells (Fig. 1 F, lane 5). Furthermore, preincubating the antibody with purified His-centrobin significantly diminished the specific signal detected by this antiserum (unpublished data). These results demonstrate that the anti-centrobin antiserum specifically detects endogenous centrobin and that centrobin is ubiquitously expressed (Fig. 1 F and not depicted).
Localization of centrobin to the centrosome
The anti-centrobin antibody characterized in Fig. 1 F was used to examine the localization of endogenous centrobin in a normal human mammary epithelial cell line (76N) and several cancer cell lines (T47D, MCF-7, and Capan-1). A typical centrosomal staining pattern was observed in all the cell lines tested, with one or two perinuclear dots in the interphase cells (Fig. 2 A, g, o, and s) and a single focus at the end of each mitotic spindle in mitotic cells (Fig. 2 A, c and k). The centrobin staining pattern was similar to that of -tubulin, a protein known to specifically localize to centrosomes (Fig. 2 A, d, h, p, and t). An identical centrosomal staining pattern was observed in MCF10A, HeLa, COS-7, and 293T cells (unpublished data). The centrosomal staining was observed under three different fixation conditions (3.7% formaldehyde, 100% methanol, or 0.5% glutaraldehyde) and also when cells were extracted with 0.5% Triton X-100 in 80 mM Pipes, 1 mM MgCl2, and 5 mM EGTA, pH 6.8, before fixation. Furthermore, the centrosomal localization of centrobin was not affected by treatment with nocodazole (unpublished data). These findings strongly indicated that centrobin is likely to be a bona fide core component of the centrosomes (Oegema et al., 1995). Importantly, GFP-centrobin and Myc-centrobin also localized to the centrosomes in the transfected cells when they were expressed at a very low level (Fig. 2, B and C). It is notable that both GFP-centrobin and Myc-centrobin formed bundle-like structures when expressed at high levels, which is probably an artifact of high-level expression because the endogenous centrobin is expressed at very low levels and is found mainly on centrosomes (unpublished data). A truncated Myc-tagged centrobin (centrobin-C; encoding the COOH-terminal 539 aa) also localized to the centrosomes when expressed at low levels (Fig. 2 D), indicating that the COOH-terminal 539 aa of centrobin is sufficient for centrosomal localization. It is noteworthy that when Myccentrobin-C was expressed at a high level it decorated the microtubules, which is also probably an artifact of high-level expression (unpublished data).
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To further characterize the localization of centrobin on the centrioles, we performed immunogold electron microscopy. Nuclearcentrosome complexes were prepared according to the Kuriyama method (Kuriyama and Borisy, 1981) and embedded in LR white resin. Thin sections were incubated with anti-centrobin antibody, followed by incubation with gold-conjugated antirabbit secondary antibodies. As in our immunofluorescence studies, centrobin clearly localized to the daughter centrioles, which are the centrioles without the characteristic appendage structure of the mother centriole (Fig. 4 D). We found that centrobin mainly localizes outside of the triplet microtubule blades of the daughter centriole (Fig. 4 D). Some centrobin staining was also found in the lumen and on the triplet microtubule blades of the daughter centriole (Fig. 4 D). Together, these results strongly indicate that centrobin preferentially localizes to the daughter centriole.
Centrobin is required for centriole duplication
We used 21-nt small interfering RNA (siRNA) targeting the coding region of centrobin to knock down centrobin expression. As shown in Fig. 5 A, the endogenous centrobin level was markedly reduced after centrobin siRNA transfection of HeLa cells, but not after the scrambled siRNA and GFP-siRNA were transfected (Fig. 5 A, top). Transfection of HeLa cells with FITC-labeled GFP-siRNA indicated a transfection efficiency of 90%. Densitometry analysis of the Western blots indicated that 80% of centrobin was reproducibly depleted with centrobin RNAi #1, which we used in all subsequent experiments. The reduction of centrobin levels was also confirmed by immunofluorescence analysis (Fig. 5 B). Immunofluorescence analysis with anti
-tubulin antibodies revealed that the
-tubulin staining pattern was not visibly altered in the HeLa cells with undetectable levels of centrobin (Fig. 5 C). Furthermore, no gross abnormalities in microtubule nucleation and organization was observed in centrobin-depleted cells (Fig. 5 D), suggesting that centrobin likely does not substantially contribute to microtubule organization and nucleation, at least in interphase cells.
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To test whether centrobin depletion directly inhibits centriole duplication, we examined the effect of centrobin depletion on HeLa cells arrested in the S phase. 48 h after siRNA transfection, the cells were exposed to HU for 24 h to induce S phase arrest. The cells were incubated for 30 min with BrdU, harvested, and stained with anti-BrdU and anti-centrobin antibodies. BrdU staining demonstrated that 94% of the control cells and 85% of the centrobin-depleted cells were arrested in the S phase, indicating that centrobin-depleted cells are still able to enter S phase (Fig. 6 D). Because centriole duplication occurs during the late G1 and S phases, all cells arrested in the S phase should contain four centrioles. Indeed, a majority (87%) of the control RNAi-transfected cells contained four centrioles (Fig. 6 E); only 9% of these cells had fewer than four centrioles. In contrast, only 48% of the centrobin-depleted cells contained four centrioles, and 50% contained fewer than four centrioles (vs. 9% of control cells; Fig. 6 E). These experiments demonstrated that the majority of centrobin-depleted cells are able to enter the S phase, but are unable to undergo centriole duplication. Therefore, the inhibition of centriole duplication upon centrobin depletion is not a consequence of cell-cycle arrest.
Furthermore, we examined the effect of centrobin depletion in U2OS cells. It has been reported that, upon prolonged S phase arrest by HU, the centrosomes in these cells become overamplified (Stucke et al., 2002). If the effect of centrobin depletion on centrosome duplication was a consequence of preventing cells from entering the S phase, then centrobin RNAi would be expected to be effective only when it was transfected into cells before HU treatment (Meraldi et al., 1999). On the other hand, if centrobin has a direct role in centrosome duplication, then centrobin RNAi would be expected to inhibit centriole duplication even when it is introduced into cells after S phase arrest. As shown in Fig. 6 F, centrosome overamplification was inhibited to a similar extent regardless of whether centrobin RNAi was introduced into U2OS cells before or after S phase arrest. We found that 52% of the cells transfected with control siRNA had overamplified centrosomes, whereas only 21% of the cells transfected with centrobin siRNA had overamplified centrosomes. Together, these findings clearly indicate that centrobin is required for centriole duplication.
Centrobin depletion leads to impaired cytokinesis
When centrobin was depleted in HeLa cells by the use of siRNA, we observed that the percentage of cells with two or more nuclei increased significantly (from 3% in control siRNA-transfected cells to 20% in the centrobin-depleted cells), indicating a failure of cytokinesis in a proportion of the centrobin-depleted cells (Fig. 7, A and B). To further explore this finding, we directly examined the progression of cell division with time-lapse microscopy. For this purpose, HeLa cells were transfected with control or centrobin siRNA. Phase-contrast time-lapse microscopy was initiated 8 h later and continued for 48 h (Videos 1 and 2, available at http://www.jcb.org/cgi/content/full/jcb.200506185/DC1). In the control cultures, 15 of the 23 observed cells completed mitosis within 2 h, and 22 of the 23 cells completed mitosis within 4 h; no cell failed to complete cytokinesis (Fig. 7, C and D). In contrast, out of the centrobin siRNA-transfected cells that went into mitosis, only 2 of 15 observed cells completed mitosis within 2 h, and only 5 of 15 cells completed mitosis within 4 h; 6 of 15 cells failed to do so within 4 h and 4 of 15 cells exited mitosis without finishing cytokinesis. This finding indicates that centrobin depletion impairs cytokinesis.
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Discussion |
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It is of particular importance that the depletion of centrobin in HeLa cells resulted in a high percentage of both interphase and mitotic cells that had two, one, or no centrioles, even under the condition of S phase arrest, which indicates that centrobin depletion inhibits the duplication of centrioles. Further analysis in U2OS cells arrested by HU treatment confirmed that inhibition of centriole duplication induced by centrobin depletion was not a consequence of cell cycle arrest. These findings have clearly established that centrobin is required for centriole duplication. The exact role of centrobin during centriole duplication remains to be determined. Because CDK2 activity has been shown to be required for centriole duplication (Hinchcliffe et al., 1999; Lacey et al., 1999; Meraldi et al., 1999), it will be of interest to examine if centrobin is a downstream target of CDK2.
We also found that -tubulin localization to the centrosomes is not visibly affected in centrobin knockdown cells. Furthermore, centrobin depletion does not appear to affect microtubule organization and nucleation visibly in interphase cells. However, we cannot exclude the possibility that centrobin plays a role in the assembly of mitotic spindles, although we did not observe any conspicuous centrobin staining on the mitotic spindles.
We have also demonstrated that the inhibition of centriole duplication by centrobin depletion leads to the lengthening of mitosis and failure of cytokinesis in a substantial population of cells. The impairment of cytokinesis induced by centrobin depletion is reminiscent of the phenotypes observed in cells when centrosomes were microsurgically removed or laser ablated (Hinchcliffe et al., 2001; Khodjakov and Rieder, 2001). In those studies, the majority of acentrosomal cells were still able to undergo mitosis but took significantly longer to complete cytokinesis, with a high percentage of cells failing to complete cytokinesis. However, the mechanism of centrobin depletioninduced impaired cytokinesis remains to be determined. Because we did not monitor the status of the centrosome in the recorded cells, we cannot differentiate the effects of centrobin directly on cytokinesis versus impaired cytokinesis because of the formation of acentrosomal spindles.
Thus, centrobin, among a few known centrosome proteins, has a particularly important function in orchestrating centriole duplication. Additional structural and functional analyses are likely to elucidate the mechanistic basis of a fundamental aspect of cell biology, namely, centrosome duplication.
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Materials and methods |
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Yeast two-hybrid constructs and screening
The cDNA encoding the COOH-terminal 1,026 residues of BRCA2 was cloned into pGBKT7 (CLONTECH Laboratories, Inc.) to generate the bait plasmid pGBKT7-BRCA2-C3. Yeast two-hybrid screening was performed as previously described (Gao et al., 1999, 2000).
Plasmid constructs and siRNA
The centrobin fragment isolated from the yeast two-hybrid library was cloned into a modified pSG5 vector, pGEX2TK, and into pPROEX Hta to generate Myc-centrobinC, GST-centrobinC, and His-centrobinC. The full-length untagged, Myc-tagged, and GFP-tagged centrobin were constructed by PCR and restriction splicing. The full-length centrobin constructs (untagged, Myc-tagged, and GFP-tagged) used in this study represent centrobin-. The centrobin-C construct used in this study contains the extra 66-bp of centrobin ß. It is referred to only as centrobin elsewhere in this paper.
The siRNAs were synthesized by Dharmacon, Inc. The sequence of centrobin siRNA #1 was AGUGCCAGACUGCAGCAACTT and the sequence of centrobin siRNA #2 was CAACUGGACAAGACCCUGGTT. The sequence of FITC-GFP siRNA was GGCTACGTCCAGGAGCGCACC and the sequence of the scrambled siRNA was CAGTCGCGTTTGCGACTGG. The siRNA transfection was performed with Oligofectamine (Invitrogen) as per the manufacturer's instructions.
Immunofluorescence
Cells grown on coverslips (Fisher Scientific) were fixed in 3.7% PFA/PBS for 10 min at RT, permeabilized in 0.5% Triton X-100/PBS, blocked with 10% goat serum in PBS, and incubated with anti-centrobin, anti-Myc (9E10), anti-tubulin, or anti
-tubulin (Sigma-Aldrich) in 10% goat serum/PBS. The primary antibodies were detected with FITC or rhodamine-conjugated goat antirabbit IgG or goat antimouse IgG (The Jackson Laboratory) and the DNA was stained with DAPI. Cells were also fixed in ice-cold methanol for 10 min, in which case the permeabilization step was eliminated. A fixation solution of 0.5% glutaraldehyde was also used. An extraction step before fixation with 0.5% Triton X-100 in 80 mM Pipes, 1 mM MgCl2, and 5 mM EGTA, pH 6.8, was added in some experiments. Gray level images were acquired using a charge-coupled device camera (model ORCA-ER; Hamamatsu) mounted on an epifluorescence microscope (Nikon) and pseudocolored using Adobe Photoshop software.
EM
For immuno-EM, centrosomenuclear complexes were enriched according to the method described by Kuriyama and Borisy (1981). In brief, 7080% confluent HeLa cells were scraped off of the culture dishes and pelleted. The cells were resuspended in 10 vol of distilled water for 1 min, an equal volume of lysis buffer (2 mM Hepes and 4% Triton X-100) was added, and the sample was incubated for an additional 5 min. An equal volume of 8% PFA plus 1% glutaraldehyde was added to fix the sample for 15 min at RT. The fixed samples were washed 3 times with Hepes buffer (20 mM Hepes, pH 7.4), dehydrated, and embedded in LR white resin (Ted Pella, Inc.). Thin sections were blocked in blocking buffer (20 mM Hepes, 1% fish gelatin, and 0.4% Triton X-100) at RT for 1 h and incubated with anti-centrobin antibody in blocking buffer (0.5 µg/ml) at 4°C overnight, followed by incubation with goat antirabbit IgG conjugated with 10-nm gold particles (Ted Pella, Inc.) for 2 h at RT. The thin sections were further stained with saturated aqueous uranyl acetate and analyzed using a transmission electron microscope (model CM-10; Philips).
To obtain serial thick sections, the purified nuclearcentrosome complexes were fixed in 2.5% glutaraldehyde for 30 min, incubated in 2% osmium tetroxide for 10 min, incubated in 2% uranyl acetate for another 10 min, and embedded in Embed 812. The samples were serially thick-sectioned at 250 or 500 nm and analyzed using a transmission electron microscope (model JEOL-1234; Japan Electron Optics Laboratory Co., Ltd.). A total of 58 centrobin knockdown cells were examined, of which 47 cells were examined using 500-nm sections and 11 cells were examined using 250-nm sections. A total of 33 control cells were examined using 500-nm sections.
Time-lapse imaging
HeLa cells plated on 35-mm dishes with glass coverslip bottoms were transfected with control siRNA or centrobin siRNA. 8 h after transfection, the medium was replaced with CO2-independent medium (Invitrogen). The cells were imaged every 5 min for 48 h using a 20x phase-contrast lens on an inverted microscope (model TE2000-U; Nikon) equipped with a charge-coupled device camera controlled by Metamorph software (Universal Imaging Corp.). The microscope is enclosed in an incubator box (Life Imaging Services) to maintain a temperature of 37°C.
Online supplemental material
Videos 1 and 2 show that cells transfected with control and centrobin siRNA underwent mitosis and that the silencing of centrobin expression leads to impairment of cytokinesis. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200506185/DC1.
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Acknowledgments |
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This work was supported by grants from the National Institutes of Health (1 R01 CA095221-01A1 and 1 R01 CA96986-01A1) and the American Cancer Society (RSG-03-048-01) to Q. Gao.
Submitted: 29 June 2005
Accepted: 4 October 2005
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