The Kelch Protein KLHDC8B Guards against Mitotic Errors, Centrosomal Amplification, and Chromosomal Instability

Background: The large multinucleated Reed-Sternberg cell is the driving force behind Hodgkin lymphoma pathogenesis. Results: Disrupting KLHDC8B function leads to multinucleation, failed mitoses, centrosomal amplification, and aneuploidy, the major pathologic features of the Reed-Sternberg cell. Conclusion: KLHDC8B protects against mitotic errors and chromosomal instability. Significance: Midbody proteins play a previously unappreciated key role in Hodgkin lymphoma pathogenesis. The malignant cell in classical Hodgkin lymphoma (HL) is the binucleated giant Reed-Sternberg cell. Chromosomal instability and mitotic errors may contribute to HL pathogenesis; one potential mitotic regulator is the kelch protein KLHDC8B, which localizes to the midbody, is expressed during mitosis, and is mutated in a subset of familial and sporadic HL. We report that disrupting KLHDC8B function in HeLa cells, B lymphoblasts, and fibroblasts leads to significant increases in multinucleation, multipolar mitoses, failed abscission, asymmetric segregation of daughter nuclei, formation of anucleated daughter cells, centrosomal amplification, and aneuploidy. We recapitulated the major pathologic features of the Reed-Sternberg cell and concluded that KLHDC8B is essential for mitotic integrity and maintenance of chromosomal stability. The significant impact of KLHDC8B implicates the central roles of mitotic regulation and chromosomal segregation in the pathogenesis of HL and provides a novel molecular mechanism for chromosomal instability in HL.

Hodgkin lymphoma (HL) 2 accounts for 11% of new lymphoma diagnoses in the United States (1). The pathologic hallmark of HL is the multinucleated giant Reed-Sternberg (RS) cell. Morphologically, RS cells are scant in number and are surrounded by nonclonal lymphocytes and other reactive cells. In recent years, the RS cell has been determined to be a B cell of germinal center origin (2,3), as demonstrated by the presence of rearranged and somatically mutated immunoglobulin variable region genes (4 -6). The multinucleated appearance of RS cells is thought to be attributable to a disturbance in cytokinesis, rather than cell fusion, by mononuclear Hodgkin cells (7)(8)(9)(10).
Some of the most conspicuous mutations in HL are chromosomal aberrations; case series show strong evidence of chromosomal instability and chromosomal aberrations in most cases of HL (11,12), where there is a particularly heavy frequency of tetraploidy or near-tetraploidy (13,14). It has been speculated that RS cells or their immediate precursors are derived from a karyotypically aberrant lineage (2). Amplification of the number of centrosomes is implicated in polyploidy in both classical HL cell lines and patient cases (15)(16)(17). Centrosomal amplification has been linked to chromosomal instability, as extra centrosomes promote chromosomal missegregation during cell division (18); such phenomena could be related to altered expression of spindle checkpoint genes (19). Telomere dysfunction in Hodgkin cells is also believed to lead to complex karyotypes and genetic instability, leading to a transition to RS cells (20,21). Nevertheless, the mechanisms underlying chromosomal instability in HL remain only partially explored.
We recently reported a candidate gene for the role of mitotic regulator in HL (22). A familial balanced translocation between chromosomes 2 and 3 resulted in classical HL occurring in several different family members due to interruption of KLHDC8B on chromosome 3, which encodes a midbody kelch domain protein expressed during mitosis. Additionally, a single nucleotide polymorphism in the 5Ј-untranslated region of the gene, which was associated with reduced translation, was also associated and linked with HL in other families. We also identified acquired loss of heterozygosity in a sporadic case of HL. Taken together, the genetic data provide compelling evidence that KLHDC8B participates in lymphomagenesis. Kelch proteins are known to facilitate protein-protein interactions and play key roles in cell division (23), yet despite the new insights from mutation of KLHDC8B, the mechanism of its function and molecular consequences of its dysfunction are unknown.
Here, we investigate the role of the HL-related protein KLHDC8B. We interfered with the function of KLHDC8B by both stable knockdown and expression of a dominant-negative KLHDC8B-GFP fusion protein. We generated multinucleated lymphoblasts that mimic the appearance of the RS cell. Video microscopy revealed the aberrant mitotic mechanisms by which multinuclear cells are generated, and we showed that loss of KLHDC8B function induces centrosomal amplification and aneuploidy, key pathologic characteristics of RS cells. Thus, we demonstrate that KLHDC8B is essential for mitotic integrity and maintenance of chromosomal stability and that loss of KLHDC8B recapitulates the major pathologic features of HL.

EXPERIMENTAL PROCEDURES
Plasmid Constructs-The tetracycline-inducible, stably transfectable anti-KLHDC8B short hairpin RNA plasmid was generated as follows. We amplified the short hairpin RNA (shRNA) from the vector TI369558 (Origene) using the forward primer 5Ј-CTTGTGGAAAGGACGCGCTCGAGTGCTG-3Ј and the reverse primer 5Ј-CACCCTAACTGACACACATTC-CACAGGG-3Ј. The shRNA segment was subcloned into the vector pSingle-tTS-shRNA (Clontech), which contains ampicillin and neomycin resistance markers. The shRNA plasmid TI369559 and noneffective GFP negative control vector TR30003 (Origene), both containing a kanamycin/puromycin selection cassette, were used without modification.
The stably transfectable expression vector for the fusion of KLHDC8B and Aequorea coerulescens GFP was generated by amplifying the cDNA of KLHDC8B with the forward primer 5Ј-TAGCTAGCCGAGGCGGAACGGCG-3Ј and the reverse primer 5Ј-GTAAGCTTGACCCCACGCAGACACAG-3Ј. The ensuing product was subcloned in-frame into pAcGFP1-N1 (Clontech), resulting in the linker peptide RILQSTVPRARD-PPV followed by the GFP domain at the C terminus of KLHDC8B.
Cell Culture-HeLa cells (ATCC) and the hTERT-immortalized human foreskin fibroblast line 82-6HT (kindly provided by P. Rabinovitch) were cultured in DMEM supplemented with 15% fetal calf serum (Invitrogen). HeLa cells were transfected using Lipofectamine and Plus reagents (Invitrogen). Stable HeLa clones were selected by plating serial dilutions and growing with medium containing 200 g/ml G418 (Invitrogen). 82-6HT cells were transfected with an Amaxa device, utilizing Nucleofector Solution V (Lonza). Stable 82-6HT clones were selected by plating serial dilutions and grown in medium containing 0.5 g/ml puromycin. Surviving colonies were harvested by trypsinizing within metal cylinders.
Antibodies, Western Blotting, and Immunohistochemistry-Chicken polyclonal IgY antibodies were raised against KLHDC8B as described previously (22). Cell extracts were prepared using a hypotonic lysis buffer supplemented with protease inhibitors (complete Mini, Roche Applied Science). Proteins were subjected to SDS-PAGE and blotted onto a PVDF membrane (Bio-Rad). Anti-KLHDC8B Western blots used a 1:10,000 dilution of primary antibody followed by a 1:10,000 dilution of horseradish peroxidase (HRP)-conjugated goat antichicken IgY secondary antibody (Aves), developed with the ECL Western blotting detection kit (Amersham Biosciences). Anti-GFP Western blots used a 1:200 dilution of rabbit polyclonal antibody SC-8334 (Santa Cruz Biotechnology), followed by a 1:5000 dilution of horseradish peroxidase (HRP)-conjugated goat anti-rabbit IgG secondary antibody SC-2054 (Santa Cruz Biotechnology), developed with the ECL kit as above. Actin loading control was detected with the C-11 HRP-conjugated antibody (Santa Cruz Biotechnology) at 1:1000 dilution.
Cell Counting and Multinucleation Analysis-HeLa and 82-6HT cells were plated at low density to coverslips, followed by formaldehyde fixation as above. Nuclei were stained with DAPI. Cells were counted manually using a Zeiss Axioplan fluorescence microscope using both fluorescence and differential interference contrast microscopy. HMy2.C1r and T5-1 lymphoblasts were cultured to a density no greater than 500,000 cells/ml, spun onto poly-L-lysine-coated slides (Thermo), and subjected to Wright staining with the Hema 3 kit (Fisher). Cells were defined as multinuclear if two or more nuclei were contained within the border of a single cell.
Live Cell Imaging-HeLa cell lines were plated at low density to 6-well plates. For live cell imaging, cells were cultured in DMEM devoid of phenol red, supplemented with 15% fetal calf serum. DNA was labeled with 0.8 M Hoechst stain for 20 min prior to imaging. Images were obtained with a Nikon TiE inverted fluorescence microscope equipped with an incubator to maintain cells at 37°C in 5% carbon dioxide. Images were recorded every 4 min over 16 -24-h periods in the differential interference contrast, GFP, and DAPI channels, with exposure times and gains adjusted to minimize exposure to ultraviolet light. Acquisition software was NIS Elements. Mitoses of mononuclear cells were considered to be aberrant if the result was anything other than two mononuclear cells. Mitoses of multinuclear cells were considered to be neither normal nor aberrant. Mitoses were considered to start with regression of the cell membrane (release of surface attachments) and were considered to end when the midbody bridge resolved or, in the case of failed cytokinesis, when the daughter cell membrane stabilized. The above timeline definitions were chosen based on the known midbody localization of KLHDC8B and its effect on multinucleation. Boundaries between mitotic phases were defined as follows: the end of prophase occurred with maximum condensation of chromosomes; the end of metaphase occurred with separation of chromosomes; the end of anaphase occurred with formation of a cleavage furrow; and the end of telophase occurred with stabilization of the nuclear membranes. We reasoned that mitotic timeline definitions based on cell sorting-measured transitions were not fully applicable to our imaging modality; furthermore, such boundaries are also fraught with subjectivity (24). The supplemental movies were generated with the Nikon Elements software package.
Karyotyping and Fluorescence in Situ Hybridization (FISH)-Cytogenetic analyses were performed with the assistance of the University of Washington Cytogenetics Laboratory. To obtain karyotypes, Giemsa banding was performed, with examination of five metaphases. For FISH, exponentially growing cells from each clone were incubated starting at a density of 4 ϫ 10 5 cells/ml at 37°C for 24 h, after which time colcemid was added to a final concentration of 0.2 mM to arrest the cells in metaphase. Cells were harvested 2 h later by centrifugation, and slides were prepared from the fixed cell suspensions. Fixed nuclei were stained with AneuVysion probes specific for chromosomes 13 and 21 (Abbott) and counterstained with DAPI.
Statistics-The p values for multinucleation assays are derived from two-tailed, two-sample t tests assuming equal variances. The p values for micronucleation and aneuploidy assays are derived from two-tailed, two-sample 2 tests using the Fisher exact test.

Stable KLHDC8B Knockdown Produces a Multinucleation
Phenotype-Patients with familial classical HL due to a balanced translocation between chromosomes 2 and 3 have haploinsufficiency of KLHDC8B, which is predicted to lead to constitutive but partial loss of protein expression. We replicated that disease scenario with stable but partial knockdown in human cell line models. We stably transfected HeLa cells with a tetracycline-inducible shRNA ("shRNA1") construct targeting KLHDC8B. Based on Western blot analysis of KLHDC8B expression, we generated two derivative cell lines with partial knockdown upon doxycycline induction (Fig. 1A). The cell lines demonstrate an increased number of multinucleated (defined as two or more nuclei) cells upon doxycycline administration ( Fig. 1, B and C) for 72 h, corresponding to ϳ3 cell generations. The effect is maintained after 144 h of doxycycline induction, suggesting that prolonged partial loss of expression leads to a stable multinucleation phenotype.
We used the same construct to stably transfect the human B lymphoblastoid cell line HMy2.C1r (25). After cloning by limiting dilution and Western blot assessment of protein expression, we produced a derivative cell line with partial KLHDC8B knockdown (Fig. 1D). As seen with HeLa, more than one band was sensitive to doxycycline induction, suggesting that the multiple bands may result from a post-translational modification. The knockdown line demonstrated increased numbers of multinucleated cells (Fig. 1E). The morphology of the multinucleated cells is reminiscent of the Reed-Sternberg cell, with copious cytoplasm and vacuolization (Fig. 1F).
KLHDC8B-GFP Fusion Protein Disrupts Cytokinesis-We sought to further explore the role of KLHDC8B in cytokinesis and multinucleation by generating a green fluorescent protein (GFP) fusion construct, suitable for in vivo cell imaging. We placed the GFP domain at the C terminus to avoid disruption of the KLHDC8B-sensitive 5Ј-untranslated region, point mutation of which influences translational efficiency and is associated with HL (22). We transiently transfected HeLa cells with an expression plasmid encoding the fusion construct of KLHDC8B and GFP (FuKG). Western blotting of lysates for both KLHDC8B and GFP confirmed the predicted protein's molecular mass of 65 kDa ( Fig. 2A). We also transfected HeLa with the same plasmid, selected for stable transfectants with G418, and we used Western blotting for GFP to select derivative lines that stably expressed FuKG.
Surprisingly, HeLa cells transiently transfected with FuKG had a multinucleation rate approximately three times greater than baseline (Fig. 2B). Confocal microscopy with immunostaining for KLHDC8B, GFP fluorescence, and DAPI staining of DNA revealed occasional post-mitotic cell pairs with agglomerations of fusion protein between daughter cells or embedded within multinucleated cells (Fig. 2C). Chromosome-like material, stained with DAPI, was stranded between the daughter cells or nuclei (supplemental Fig. 1). Thus, FuKG has the unanticipated ability to interfere with midbody function and appears to function as a dominant-negative form of KLHDC8B, in the sense that it disrupts function by the presence of small quantities that antagonize the normal function of the wild-type protein.
We generated stably transfected HeLa lines expressing FuKG to better explore the mitotic effects of interfering with KLHDC8B's function. Stable expressors of FuKG were selected by Western blot screening of cell lysates for KLHDC8B and GFP ( Fig. 2A). Stable transfectants expressed lower quantities of FuKG protein than transient transfectants. We surmised that high levels of FuKG expression were toxic and interfered with cell line viability. Stable expression of FuKG (clones 10 and 19) induced the highest rates of multinucleation that we had observed, up to 14%. As controls, we utilized untransfected HeLa and derivative clones (clones 1 and 22) that demonstrated G418 resistance but no detectable FuKG expression by Western blot (Fig. 2D). Confocal imaging of the stable expressors once again revealed the presence of fusion protein aggregates (Fig. 2E). We found that the presence of GFP-fluorescing aggregates was statistically associated with the characteristics of multinucleation (Table 1), supporting the argument that interfering with KLHDC8B function contributes to multinucleation. Our imaging experiments uncovered an increased presence of micronuclei in cell lines expressing FuKG, suggesting that the fusion protein additionally contributes to missegregation of chromosomes (Table 2).
To assess the impact of KLHDC8B on the mitotic spindle, we performed confocal imaging with immunofluorescence directed against ␣-tubulin. Stable FuKG expressors showed fraying of microtubules and an increased propensity to form multipolar spindles, although inadequate numbers of spindles were available for statistical analysis (supplemental Fig. 2).
We performed live cell fluorescent video microscopic observations of the two FuKG stable transfectant lines to explore how the dominant-negative fusion protein caused multinucleation. Three control cell lines were utilized (two FuKG nonexpressors and untransfected HeLa) to evaluate for the effects of UV expo-sure and DNA labeling on cell division. We did not observe any cell fusion events for the expressor lines FuKG10 (n ϭ 375) or FuKG19 (n ϭ 283), supporting our working hypothesis that KLHDC8B disruption induces multinucleation through disruption of cytokinesis. We defined aberrant mitoses of mononuclear cells as those resulting in an outcome other than two mononuclear daughter cells (Fig. 3A). The FuKG expressor lines demonstrated increased rates of aberrant mitoses compared with nonexpressor and untransfected controls (Fig. 3B). Peri-mitotic blebbing was a frequent observation in expressor cell lines. Among aberrant mitoses, failed abscission events (inability to initiate or complete a cleavage furrow) were most common; there were also high rates of anucleate cell generation and multipolar mitoses, occasionally with generation of three daughter cells (Table 3 and supplemental . FuKG expressors demonstrated a longer average duration of mitosis, with abnormal mitoses accounting exclusively for the difference in the length of time required to complete mitosis (Fig. 3C). This suggests that the abnormal mitoses induced by the fusion protein are qualitatively different somehow from mitotic errors that would be present at baseline. We arbitrarily culled 62 mitoses (29 normal, 33 aberrant) from two separate live cell imaging experiments on line FuKG10 for detailed analysis of mitotic phase times. We found that prophase, metaphase, and anaphase were not statistically prolonged for aberrant mitoses. However, cytokinesis duration was roughly tripled, and telophase demonstrated a statistically significant but minor prolongation (Fig. 3D). Among the 33 aberrant mitoses, the phase of failure was distributed as follows: cytokinesis 16, telophase 10, anaphase 6, and metaphase 1.
Although FuKG expressor lines produced only small amounts of fusion protein, we recorded several instances of perimitotic fusion protein expression accompanied by aberrant mitoses (supplemental Fig. 3 and supplemental movie 6). Taken together, the results suggest that KLHDC8B is a key component     NOVEMBER 9, 2012 • VOLUME 287 • NUMBER 46 of midbody function, affecting not just abscission but also appropriate chromosomal and nuclear segregation.

KLHDC8B-GFP Fusion Protein Induces Centrosomal
Amplification-Induction of tripolar mitoses and anucleate daughter cells suggested that KLHDC8B influences centrosome function. Therefore, we asked whether expression of the FuKG protein could induce centrosomal amplification. We assessed centrosome number and architecture by performing immunohistochemistry studies on stable HeLa expressors of FuKG, using antibodies against pericentrin, a centrosomal protein commonly used to visualize centro-somes. Control cell lines were the same as those used for the multinucleation and live cell imaging assays. The cell lines expressing the FuKG protein demonstrated marked increases in the number of cells with centrosomal amplification (three or more centrosomes) compared with controls (Fig. 4A). Among the cells with centrosomal amplification, three was the most common number; it is notable that even numbers of centrosomes were not predominant (Fig. 4B). We did not observe significant alterations in centrosomal architecture such as enlargement. Centrosomal amplification was strongly correlated with multinucleation, and  greater numbers of nuclei appeared linked with greater numbers of centrosomes, although the size of the sample was inadequate for statistical analysis. However, expressor lines demonstrated an elevated incidence of centrosome amplification even in mononuclear cells (Table 4). Fig. 4, C and D, demonstrates centrosomal amplification in expressor lines, including a metaphase notable for three centrosomes and FuKG expression. Stable KLHDC8B Knockdown Induces Aneuploidy-To investigate whether KLHDC8B protects against chromosomal instability, we sought diploid but transfectable and clonable cell lines. The B lymphoblastoid line T5-1 and the human foreskin fibroblast line 82-6HT met our requirements, with minor deviations from otherwise diploid karyotypes as follows: 46,XY,t(6; 11)(p11;p11.1) for 82-6HT and 46,X,-X or -Y,dup(7)(q11.2q32) for T5-1. To confirm the knockdown phenotype, we determined whether T5-1 and 82-6HT would also be vulnerable to multinucleation after knockdown of KLHDC8B. For cytogenetic experiments, we utilized a puromycin-selectable, constitutively expressed shRNA ("shRNA3") with a more potent knockdown effect than the shRNA1 we used above, as shown previously by Salipante et al. (22). Stable transfectant clones of T5-1 and 82-6HT were derived and screened for KLHDC8B knockdown by Western blotting (Fig. 5A). We analyzed two lines each from T5-1 and 82-6HT that displayed increased multinucleation (Fig. 5B). Furthermore, immunostaining demonstrated that the two fibroblast lines have centrosomal amplification (supplemental Fig. 4).
We assessed chromosome segregation abnormalities by performing interphase FISH on chromosomes 13 and 21. Both chromosomes are acrocentric, and we reasoned they might undergo nondisjunction events at higher frequency. Chromosome numbers were assessed per nucleus, rather than per cell, as the protocol involved cell lysis. Among T5-1 cells, knockdown lymphoblast clone 1 (KL1) demonstrated statistically significant increased numerical abnormalities for chromosomes 13 and 21 individually. Abnormalities ranged from absence of a chromosome to the presence of as many as seven copies of a particular chromosome. Knockdown lymphoblast clone 2 (KL2) trended toward an increase in numerical chromosomal abnormalities. For both lines, numbers of nuclei with tetrasomy of either chromosome were statistically significant, with a ratio of 3:1 for knockdown to control. Among 82-6HT, knockdown fibroblast clone 2 (KF2) demonstrated statistically significant increased numerical chromosomal abnormalities, with tetrasomy for either chromosome 13 or 21 being the most commonly seen aberration; other abnormalities of number were also observed, but no cell had more than four copies of either chromosome. Knockdown fibroblast line 1 (KF1) did not demonstrate an increase in numerical aberrations by FISH (Fig. 5C). Thus, in three of the four diploid cell lines evaluated, across two different cell types, there was statistically significant induction of aneuploidy caused by depletion of KLHDC8B. Notably, the propensity for tetrasomy appears to correlate with tetraploidy and near-tetraploidy as common cytogenetic abnormalities in HL.

FIGURE 4. Expression of FuKG induces centrosomal amplification.
A, fusion protein expressors and control lines were plated to coverslips at low density and grown for 48 h. Anti-pericentrin immunofluorescence was used to determine the number of centrosomes per cell. Cells with three or more centrosomes were considered to be have centrosomal amplification. 600 cells were counted for each line, with the exception of HeLa (n ϭ 800). Fusion protein expressors FuKG10 and FuKG19 demonstrated significant centrosomal amplification. B, centrosomally amplified cells were categorized by the number of centrosomes in each cell. Greater numbers of centrosomes were associated with decreasing numerical frequency, suggesting that centrosomal amplification is not merely the result of duplication secondary to failed abscission events. C, representative cell with centrosomal amplification. The inset shows the differential interference contrast image of this binucleate cell. Confocal microscopy shows the staining for pericentrin (red) and DNA (blue), with expression of fusion protein (green) also present. The image shown is the composite overlay of a Z-stack of images. D, FuKG expressor cell with three centrosomes present at metaphase, rather than the expected two. Staining performed as in C. There is expression of fusion protein at the time of mitosis. Notably, centrosomal amplification is present prior to completion of mitosis.

DISCUSSION
The RS cell, of germinal center B lymphocyte origin, is the malignant cell of HL (2,3). By interfering with the function of the midbody protein KLHDC8B, we reproduced the major pathologic features of the RS cell as follows: multinucleation, defective cytokinesis, centrosomal amplification, and aneuploidy. Using shRNA knockdown of KLHDC8B, we generated multinucleated B lymphoblasts that are morphologically similar to RS cells; we also induced aneuploidy, in particular tetraploidy, in B lymphoblasts and fibroblasts by means of KLHDC8B knockdown. Expression of the dominant-negative KLHDC8B-GFP fusion protein resulted in defective cytokinesis, with multiple instances of failed abscission, generation of anucleate daughter cells, and multipolar mitoses, providing potential mechanistic explanations for how RS cell morphology might arise. The presence of these alterations in several different derivative lines from multiple cell types, also seen in the FuKG cell lines, reinforces the validity of the findings and strongly argues against an off-target shRNA effect. The multinucleation data and live cell imaging provide evidence supporting the long held hypothesis that defective cytokinesis, rather than cell fusion, is responsible for the appearance of the RS cell (8,9). Our data suggest that disruptions of mitotic mechanics play a central role in the pathogenesis of HL.
Aneuploidy, especially tetraploidy, and other chromosomal abnormalities are well documented in HL, pointing toward chromosomal instability as an underpinning of HL pathogenesis (11,12,16,26). We present data suggesting that deficiency or malfunction of a midbody protein, in this case KLHDC8B, leads to failed cytokinesis and centrosomal amplification. In turn, centrosomal amplification increases the propensity of cells to missegregate individual chromosomes and perhaps even entire sets of chromosomes (i.e. nuclei). The results described were not limited to lymphoid cells, suggesting that the mechanism for chromosomal instability in HL may also be applicable to a variety of malignant and nonmalignant diseases characterized by defective midbody function. Interestingly, disruption of normal telomere length has also been shown to lead to similar anucleate cells in HL cell lines and is implicated in the transition from the Hodgkin cell to the RS cell, suggesting an alternate mechanism for mitotic errors that might lead to formation of the RS cell (20,21,27).
The KLHDC8B-GFP fusion protein (FuKG) appears to function as a dominant-negative mutant. The GFP fusion protein induces multinucleation more potently than depletion of KLHDC8B by RNAi. Stable transfectants, which produce small amounts of FuKG protein relative to native KLHDC8B, have a

KLHDC8B Prevents Chromosomal Instability
profound effect on multinucleation and centrosomal amplification, presumably due to prolonged expression of the protein under selection pressure. Expression of FuKG replicates the effects of RNAi-mediated depletion of KLHDC8B, most notably multinucleation and centrosomal amplification, although it is not certain whether the effects of protein depletion and FuKG expression operate by the same mechanism. Occasional midbody localization of FuKG and perimitotic expression of FuKG support the notion of the dominant-negative role of FuKG. The fusion protein may interfere with normal functions of KLHDC8B. Those findings also suggest the possibility that aggregates of FuKG in the midzone region cause steric interference. There is recent evidence that dominant-negative mutations occur naturally in some types of kelch proteins and can be disease-causing; one example is KBTBD13, which is linked to nemaline rod myopathy (28). KLHDC8B is one of 71 known or predicted human "kelch" family genes (29). Kelch proteins contain five to seven repeats of the ϳ50-amino acid kelch motif, coming together to form a ␤-propeller configuration (23); most kelch proteins contain additional domains, such as a "BTB/POZ" domain. KLHDC8B is one of only two kelch proteins containing seven kelch repeats and one of only seven lacking other recognizable domains. Kelch proteins participate in diverse biochemical activities, but a unifying theme is widespread participation in the machinery of cytokinesis (30). Participation in cytokinesis may be linked to the kelch domain's recognized ability to bind actin and participate in protein-protein interactions; the biochemical interactions of KLHDC8B are an intriguing topic for future exploration. KLHDC8B may not be unique in contributing to proper lymphoid development; the closely related BTB-kelch protein KLHL6 is necessary for B cell receptor signaling and germinal center formation (31).
Our results clarify the role of KLHDC8B in mitosis. KLHDC8B contributes to proper completion of abscission; this is consistent with our frequent video microscopic findings of failure to initiate or complete cleavage furrows. KLHDC8B may also contribute to the appropriate delivery of daughter nuclei to daughter cells, as evidenced by the significant number of anucleate cells generated by aberrant mitoses. Another kelch protein that localizes to the midzone, KLHL21, appears to be required for cytokinesis as well (32). BRCA2, most famous for its role in DNA damage control in the nucleus, localizes to the midbody; cell lines deficient in BRCA2 have difficulty completing cytokinesis and an increased fraction of binucleate cells (33). Thus, there is precedent for the behavior of KLHDC8B among midbody proteins. These observations are consistent with the hypothesis of Harvey (34) that binucleate cells arise by the failure of cell division after nuclear division. Cytokinesis failure alone increases the risk for tumorigenesis, due to the creation of tetraploid cells that are prone to chromosome missegregation and chromosomal rearrangements (35).
We observed a longer aggregate duration of mitosis with the dominant-negative protein FuKG. This delay, which is confined to cells undergoing aberrant mitoses, suggests activation of a checkpoint during mitosis (24). One example is the "mitotic checkpoint" during the metaphase-anaphase transition, which is triggered by unattached kinetochores and can delay anaphase for several hours (36). However, delayed or failed resolution of the midbody bridge accounts for the majority of the prolonged mitoses in our study. Similar outcomes have been demonstrated with depletion of BRCA2; multinucleated cells result, and cytokinesis is delayed (33,37).
KLHDC8B plays a role in maintaining mitotic integrity, which likely is responsible for the findings of missegregation of chromosomes and even entire nuclei, which can occur in the presence of the dominant-negative FuKG. Other kelch domaincontaining proteins may play similar roles. Keap1 appears to have a significant function in the midbody, where it locates during cytokinesis. RNA interference of Keap1 has been shown to contribute to multinucleation and chromosomal segregation defects in Caenorhabditis elegans (38). KLHL21 has been shown to associate with the chromosome passenger complex and aurora B (32), supporting the notion that different midbody kelch proteins can play essential roles in spindle checkpoint regulation and maintenance of chromosomal stability. As KLHDC8B lacks other recognizable functional domains (29), its range of intermolecular interactions may be more limited than those of BTB-Kelch proteins. Centrosome amplification has been described in a variety of solid tumor and hematologic malignancies (39). Our results strongly imply that impaired midbody function or missing spindle checkpoint regulators can lead to centrosomal amplification in HL, although the mechanisms require further elucidation. Previous studies have also suggested that centrosomal amplification may arise independently of mitotic failure. It has been proposed that increased even numbers of centrosomes (i.e. 4, 6, 8, etc.) imply that mitotic failure is the driving force behind centrosomal amplification (40). We observed odd numbers, with three being predominant, in addition to even numbers (Fig. 4B), suggesting that KLHDC8B may have an impact on centrosome number outside of mitotic failure; a similar observation was made with centrosome amplification in endothelial cells (41). Nevertheless, KLHDC8B also seems to make a significant contribution to centrosomal amplification due to abscission failure, as centrosome number appeared correlated with multinucleation. Supernumerary centrosomes are known to cause multipolar mitoses and chromosome missegregation (18,40,42), suggesting a direct link between centrosome amplification and chromosomal instability, both of which are observed in our cell line models. We did find that multipolar mitoses were increased in the FuKG fusion protein expressors but were not present in large numbers. Malignant cells often have extra centrosomes but likely suppress multipolar mitoses as part of their survival strategy (43).
The strongest link between KLHDC8B and malignant transformation is the induction of aneuploidy upon knockdown. The estimated baseline rate of aneuploidy in human primary cells is about 0.01 per cell (44); the base-line rates of aneuploidy in our controls were roughly similar (0.005 per fibroblast and 0.02 per lymphoblast). KLHDC8B knockdown produced an approximate doubling in the numerical abnormalities of individual chromosomes. The increase was consistent across three cell lines in two different cell types and mirrors the increase in multinucleation seen with KLHDC8B depletion. Furthermore, increased rates of chromosomal aberrations such as aneuploidy KLHDC8B Prevents Chromosomal Instability NOVEMBER 9, 2012 • VOLUME 287 • NUMBER 46 and micronuclei are associated with increased risk of cancer (45). Aneuploidy due to either loss or overexpression of spindle checkpoint proteins has been linked to tumorigenesis in studies of the kinetochore-localized protein kinases BUB1 and BUB1B (46,47). In addition, the most common cytogenetic abnormality induced by KLHDC8B knockdown, tetrasomy, correlates with the tetraploid changes frequently seen in HL (13,14). Findings of aneuploidy in response to KLHDC8B knockdown are thus consistent with results from other midbody proteins, although midbody proteins may impact chromosomal stability by playing roles that extend beyond regulation of abscission.
The accumulation of whole-genome sequencing data from individual malignancies has led to the identification of major pathways susceptible to tumor-inducing mutations (48). Twelve major groups of genes were referenced in the initial study. We suggest that mitotic and spindle checkpoint proteins should also be considered one of the key susceptible pathways, as demonstrated by the mounting body of evidence elucidating the roles of kelch and other functionally analogous proteins (30). Continued study of proteins such as KLHDC8B is demonstrating how genes encoding the cytokinetic machinery contribute to faithful cell division and segregation of chromosomes. KLHDC8B and other midbody proteins represent a significant category of albeit underappreciated tumor suppressors; the revelation of their mechanisms of action continues to bear out the hypotheses laid down many decades ago by pioneers such as Boveri (49) and Harvey (34).