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Fox Chase Cancer Center, Philadelphia, Pennsylvania 19111,1 University of Pennsylvania, School of Veterinary Medicine, Philadelphia, Pennsylvania 191042
Received 1 September 2006/ Returned for modification 19 October 2006/ Accepted 30 October 2006
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ABSTRACT |
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INTRODUCTION |
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Information that is not directly coded by the DNA sequence but instead is encoded by DNA methylation, histone modifications, or other aspects of chromatin structure, is epigenetically determined. The histone modifications that contribute to epigenetic information have been proposed to constitute a histone code, by analogy to the genetic code (68). Cells possess elaborate mechanisms to sense and repair damage to the genetic code (19). Extending the analogy between the genetic code and the histone code, if histone and DNA modifications encode information outside of the DNA sequence, the cell is likely to have mechanisms to sense and repair, or otherwise respond to, alterations in these modifications. How cells respond to alteration of chromatin and epigenetic modifications is poorly understood.
Kinetochores are large macromolecular protein assemblies on chromosomes (31) that serve as attachment sites for the spindle microtubules that pull apart the sister chromatids during mitosis. Foundation proteins—CenpA, CenpB, CenpC, CenpH, CenpI, and hMis12—set the location of the kinetochores. These proteins form the base of the kinetochore complex that ultimately includes proteins required for the initiation, maintenance, and monitoring of microtubule attachments, as well as suppression of chromosome segregation until all attachments are properly formed (31). Depending on the specific chromosome, human kinetochores are built on hundreds to thousands of kilobases of repetitive centromeric 
-satellite DNA. Flanking these -satellite repeats are additional extended repeat sequences, pericentromeric DNA. Pericentromeric repeats contain -satellites, 
-satellites, satellite III sequences, and interspersed L1 LINE retrotransposons. Despite the sequence similarity underlying kinetochores, the existence of neocentromeres—fully functional kinetochores at noncanonical sites with no DNA sequence similarity to canonical centromeres—indicates that the assembly of kinetochores is primarily defined by the chromatin structure and not DNA (31).
Recent studies have defined a direct link between kinetochore assembly and function and the underlying chromatin structure. The pericentromeric DNA repeats that flank the centromeric -satellite DNA are incorporated into compact constitutive heterochromatin. This pericentromeric heterochromatin contains specific histone modifications, such as a high level of methylated lysine 9 of histone H3 (H3K9Me) and low levels of acetylated lysine 9 of histone H3 (H3K9Ac) and methylated lysine 4 of histone H3 (H3K4Me) (31). In addition, pericentromeric heterochromatin is enriched in a family of low-molecular-weight proteins—HP1, HP1ß, and HP1—that bind to heterochromatin through an interaction with H3K9Me of heterochromatin and/or through the histone variant H2AZ (49) and/or an unknown RNA component (3, 18, 24, 32, 37). HP1 proteins are thought to contribute to the transcriptional silencing of heterochromatin (39, 41, 50, 53). In addition, HP1 proteins at pericentromeres physically interact with the kinetochore foundation protein, hMis12. Consequently, HP1 proteins are required for the recruitment of hMis12 to kinetochores and also to suppress formation of aberrant micronuclei which are thought to result from defective chromosome segregation in mitosis (40).
In recent years, much has been learnt of the mechanisms that protect a cell's genetic integrity, from studies with radiation and small molecules, such as hydroxyurea, aphidicolin, and methyl methanesulfonate, which induce genotoxic stress (19). In an analogous fashion, we investigated here the response of primary human cells to a panel of small molecules that disrupt DNA and histone modifications and, presumably, epigenetically encoded information. Specifically, we have utilized several histone deacetylase inhibitors and an inhibitor of DNA methylation, all of which antagonize formation of heterochromatin (25). In response to perturbation of heterochromatin by these small molecules, primary human cells mount a dynamic mobilization of HP1 proteins to further enrich these proteins at the pericentromeric regions. Relocation of these proteins depends upon deposition of the histone variant H3.3 in the pericentromeric chromatin, mediated by the histone chaperone HIRA. Although inactivation of HP1 proteins on their own had no detectable effect on the cells, simultaneous perturbation of heterochromatin with small molecules and inactivation of HP1 proteins caused gross defects in kinetochore structure. Specifically, kinetochores were depleted of the HP1-binding protein, hMis12. Ultimately, these cells died after aberrant progression through mitosis, with defects characteristic of defective kinetochore function. We conclude that perturbation of epigenetic heterochromatin modifications causes dynamic recruitment of HP1 proteins to pericentromeres, so as to maintain kinetochore structure and function through the recruitment of hMis12 to kinetochores. These results indicate that HP1 proteins are essential players in a dynamic "repair-like" response to perturbation of heterochromatin that preserves the functional integrity of heterochromatin.
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MATERIALS AND METHODS |
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FACS, TUNEL, immunofluorescence, and immunofluorescence-fluorescence in situ hybridization (FISH).
Fluorescence-activated cell sorting (FACS) and TUNEL (terminal deoxynucleotidyltransferase-mediated dUTP-biotin nick end labeling) assays were performed as previously published (15). Anti-HP1 was a gift from William Earnshaw. Anti-HP1ß (Chemicon), anti-HP1 (Chemicon), anti-H3 (Upstate), and anti-acetyl-H3 (Upstate) were from the indicated suppliers. Anti-Bub1 and anti-macroH2A antibodies have been described previously (9). Anti-hMis12 antibody was raised in rabbit by using purified hMis12 protein as described previously (40). ACA antibody was a gift from J. B. Rattner, University of Calgary. Two- and three-color immunofluorescence was performed as described previously (74).
Immunofluorescence-FISH was performed as previously described (55). Briefly, after regular immunostaining, slides were fixed in 4% paraformaldehyde in phosphate-buffered saline for 10 min at room temperature and washed three times with double-distilled H2O and then further fixed in methanol-acetic acid (3:1) for 15 min at room temperature. The slides were dehydrated by sequential immersion in 70, 90, and 100% ethanol at room temperature for 2 min for each treatment, followed by complete drying of the slide at room temperature. The DNA was denatured by immersion of the slides in 83°C 70% formamide in 2x SCC (1x SSC is 0.15 M NaCl plus 0.015 M sodium citrate) for 4 min, followed by dehydrating the slides immediately in –20°C 70, 90, and 100% ethanol (2 min for each treatment). The slides were then dried completely at room temperature. The pericentromeric satellite III probe was PCR amplified from genomic DNA using 5'-TCCCTTTCGAGTCCATTCAATG-3' (forward) and 5'-GATCATCATCGAATGGACCC--3' (reverse) primers with Pfu polymerase and biotin labeled with Bioprimer DNA labeling kit (Invitrogen). The probe was dissolved in 50% formamide in 2x SSC solution and hybridized overnight at 37°C. After hybridization, the slides were washed once in 50% formamide in 2x SSC for 15 min at 43°C, followed by two washes in 2x SSC for 5 min each time at room temperature. The signal was detected by avidin-fluorescein isothiocyanate (Vector Laboratories) binding and amplified by biotinylated anti-avidin (Vector Laboratories), followed by another layer of avidin-FITC.
Image collection was done by examining optical sections obtained with a confocal microscope or digital images obtained using an epifluorescence microscope and a cooled charge-coupled device camera. The details of these procedures are available on request.
ChIP analysis.
Chromatin immunoprecipitation (ChIP) analyses were performed as described previously (43). Cross-linking was performed with 1% formaldehyde. For each immunoprecipitation, 10 µg of antibody was used to immunoprecipitate sonicated chromatin from 5 x 105 cells. The anti-HIRA (D34 and WC15) antibodies were as described previously (15). Anti-HP1 (Upstate), anti-acetyl-H3 (Upstate), anti-H3K9Me2 (Abcam), anti-H3K9Me3 (Abcam), anti-H3 (Abcam), and anti-HA (Y11; Santa Cruz) antibodies were from the indicated suppliers. The PCR primer sequences for pericentromeric repetitive satellite III were 5'-TCCCTTTCGAGTCCATTCAATG-3' (forward) and 5'-GATCATCATCGAATGGACCC--3' (reverse). PCR was performed with Pfu polymerase (Stratagene).
siRNAs, nucleofection, and retroviruses.
All small interfering RNAs (siRNAs) were purchased from Dharmacon. The sequences were as follows: siHIRA#2, sense strand, 5'-GGAGAUGACAAACUGAUUAUU-3'; siHIRA#4, sense strand, 5'-GAAAUUCUAGCUACUCUGAUU-3'; siH3.3A, sense strand, 5'-CUACAAAAGCCGCUCGCAAUU-3'; and siH3.3B, sense strand, 5'-GCUAAGAGAGUCACCAUCAUU-3'. Nucleofection of siRNAs, pBos-H2B-GFP, and pBCHGN-GFP-HP1 was performed according to the manufacturer's instructions (Amaxa Biosystems). The following plasmids were used to generate retroviruses: pQCXIP-H2B-GFP, pQXCIP-HA-HP1ß(103-185) (HP1ß
N), pQCXIP-HA-HP1ß, pQCXIP-HA-H3.1, and pQCXIP-HA-H3.3. Retrovirus-mediated gene transfer was performed as described previously (74), using Phoenix cells to make the infectious viruses (Gary Nolan, Stanford University). Virus infections were performed at a multiplicity of infection of approximately 1.
Live cell imaging. H2B-green fluorescent protein (GFP) was expressed in WI38 cells by nucleofection or retrovirus-mediated gene transfer. Cells were seeded the day before imaging. Two hours before imaging, the medium was changed from regular Dulbecco modified Eagle medium to phenol-free and HEPES-buffered Dulbecco modified Eagle medium. HDIs were added at the indicated time prior to imaging. Immediately prior to imaging, the surface of the medium was covered by mineral oil. Images were acquired automatically at multiple locations by using an inverted Nikon TE2000 microscope fitted with a x10 Plan Fluor objective lens using a Cascade 650 monochrome camera (Photometrics). The microscope was housed in a 37°C chamber. Fluorescence and differential interference contrast images were obtained every 10 min for a period of 24 to 36 h. The images were acquired and processed by using MetaMorph software (Universal Imaging/Molecular Devices). Scale bars were set at 10 µm.
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RESULTS |
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fused to GFP at its N terminus in WI38 cells. In the absence of HDIs, GFP-HP1 was enriched in some large foci at unknown sites that did not colocalize with ACA. However, HDIs caused GFP-HP1 to colocalize with ACA, similar to the endogenous proteins (Fig. 2B). FRAP analysis showed that the GFP-HP1 recruited to foci by TSA was more stably bound to chromatin than GFP-HP1 in the bulk nucleoplasm (data not shown), a characteristic of heterochromatic HP1 proteins (7). We also showed by double-label immunoFISH analysis that TSA treatment of WI38 cells caused the relocalization of HP1ß to pericentromeric sequences, the latter defined by their hybridization to a pericentromeric satellite III probe (Fig. 2C). Moreover, ChIP analysis of endogenous, untagged HP1 also showed that this protein is recruited to repetitive pericentromeric satellite III DNA sequences in response to HDIs (Fig. 2D and see Fig. S2 in the supplemental material).
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Recruitment of HP1 proteins depends on histone chaperone HIRA and histone variant H3.3. Next, we set out to determine the mechanism by which HP1 proteins are recruited to pericentromeres. Previously, we found that the histone chaperone, HIRA, drives the formation of domains of heterochromatin, SAHF, in senescent human cells (74). Significantly, HIRA's role in heterochromatin formation is conserved through evolution (4, 12, 20, 21, 46, 59, 74). Moreover, the orthologs of human HIRA in Saccharomyces cerevisiae and Schizosaccharomyces pombe are required for proper centromeric and pericentromeric chromatin structure, respectively (4, 60). In light of these observations, we sought to determine whether CDA-induced recruitment of HP1 proteins to pericentromeres in human cells depends on HIRA. First, we used a dominant-negative HIRA mutant to inhibit HIRA activity. This N-terminal truncation mutant, HIRA(520-1017), was fortuitously identified by virtue of its ability to block formation of SAHF in senescent human cells (X. Ye, B. Zerlanko, R. Zhang, N. Somaiah, M. Lipinski, and P. D. Adams, submitted for publication). When this mutant protein was expressed in WI38 cells, it blocked the recruitment of HP1 proteins to pericentromeres in response to CDAs (Fig. 3A and B). To more rigorously test whether HIRA is required for this response, we knocked down HIRA in WI38 cells using two different siRNAs targeted to HIRA. Knock down of HIRA did not affect the total abundance of endogenous HP1 proteins (data not shown) but did block their relocalization to pericentromeres (Fig. 3C and D). There was no effect of a control siRNA, confirming that HIRA is necessary for CDA-induced recruitment of HP1 proteins to pericentromeres.
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The histone chaperone HIRA is known to favor the histone variant, histone H3.3, as a deposition substrate (63). Therefore, we sought to determine whether CDAs induce deposition of this histone variant into pericentromeres and whether this is required for recruitment of HP1 proteins. Since histone H3.3 and the canonical histone H3.1 are not immunologically distinguishable, to determine whether CDAs induce deposition of histone H3.3 and/or histone H3.1 at pericentromeres we ectopically expressed HA-tagged histone H3.3 or histone H3.1 in WI38 cells, treated the cells with TSA, and then performed ChIP analysis with an anti-HA antibody and scored for the coprecipitation of satellite III sequences. TSA induced a striking recruitment of HA-tagged histone H3.3 to pericentromeres and a reciprocal depletion of canonical histone H3.1 (Fig. 4A). Significantly, histone H3.3 was recruited to pericentromeres before HP1, a finding consistent with the proposal that the deposition of histone H3.3 is required for the recruitment of HP1 (compare Fig. 2D and 4A and see also Fig. S2 in the supplemental material). To directly ask whether recruitment of histone H3.3 is required for recruitment of HP1 proteins to pericentromeres, we used two siRNAs to simultaneously knock down the endogenous products of the two genes coding for histone H3.3, H3.3A, and H3.3B, without affecting canonical histone H3.1 (Fig. 4B). Strikingly, an 
50% knock down of histone H3.3 mRNA resulted in a 50% block to the recruitment of HP1 proteins to pericentromeres after TSA treatment (Fig. 4C and D). We conclude that the preferred substrate of the histone chaperone HIRA, histone H3.3, is also required for the recruitment of HP1 proteins to pericentromeres and the deposition of histone H3.3 occurs, directly or indirectly, via its exchange with histone H3.1.
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N) was generated and stably, ectopically expressed in WI38 cells by retrovirus infection and drug selection. As predicted, the amount of all three chromatin-bound endogenous HP1 isoforms was reduced by ca. 80% based on immunofluorescence and Western blot assays, indicating that this mutant functions efficiently as a dominant-negative mutant (Fig. 6A and B). Remarkably, stable ectopic expression of HP1ßN had no effect on the cell growth, viability, or life span of primary human fibroblasts (Fig. 7A, B, and D and data not shown). The apparent lack of any phenotype in these cells might be because the residual 20% of chromatin-bound HP1 proteins is sufficient to mediate all essential HP1 functions under unstressed conditions. Regardless, if CDA-induced relocalization of HP1 proteins reflects an essential dynamic protective function of these proteins in the presence of altered heterochromatin modifications, HP1 proteins ought to be essential in the presence of CDAs.
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N mutant to determine whether functional HP1 proteins protect cells from the debilitating effects of HDIs. Control primary human fibroblasts or the same cells stably expressing HP1ßN were treated with or without TSA. After TSA treatment, HP1ßN failed to localize to pericentromeres itself and blocked the relocalization of endogenous HP1 proteins (Fig. 6C). Strikingly, the hMis12 signal at kinetochores was almost completely abolished in the TSA-treated HP1ßN-expressing cells, below the level observed with TSA alone (Fig. 6D and 1E). Moreover, compared to the control cells, cells expressing HP1ßN and unable to recruit HP1 to pericentromeres were exquisitely sensitive to killing by HDIs (Fig. 7A). HDI-treated HP1ßN-expressing cells died by apoptosis, as judged by the presence of sub-G1-phase and TUNEL-positive cells (Fig. 7B and C). To test whether cell killing was a consequence of extreme defects in mitotic progression, in other words a worsening of the defects seen with TSA alone (Fig. 1), the cells stably expressing HP1ßN were infected with a retrovirus encoding H2B fused to GFP at its C terminus and then treated with or without TSA. Consistent with the apparently normal growth of the HP1ßN-expressing cells in culture (Fig. 7A, B, and D and data not shown), mitosis in these cells in the absence of HDIs was indistinguishable from the control cells; in both cases cells completed mitosis in about 40 min (Fig. 7Di and ii). As shown previously, the TSA-treated control cells also completed mitosis, even though they took more than 1 h to do so and exhibited some unaligned and lagging chromosomes in the process (Fig. 1D and 7Diii). In stark contrast, the TSA-treated HP1ßN-expressing cells typically failed to progress from prometaphase to metaphase, and then, after a long delay of several hours, returned to interphase, often losing chromosomes in the process and eventually dying from apoptosis (Fig. 7Div and v). Together, these data show that disruption of HP1 protein function worsens the HDI-induced defects in kinetochore structure, as indicated by a complete loss of hMis12, and prevents alignment of chromosomes at the metaphase plate, ultimately causing an aborted mitosis and cell death. The fact that WI38 cells stably expressing HP1ßN exhibited no detectable defects when repeatedly analyzed over 20 to 30 population doublings shows that the profound effect of TSA on these cells is not due to worsening of a phenotype that already exists at low level in the HP1ßN cells. We conclude that, in the presence of HDIs, recruitment of HP1 proteins to pericentromeres maintains the levels of hMis12 at kinetochores and protects cells from the lethal damaging effects of HDIs. |
DISCUSSION |
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Our finding that HDIs induce localization of additional HP1 proteins to pericentromeres is in apparent contrast to previous studies, which showed that HDIs cause a depletion of HP1 proteins from pericentromeres (8, 51, 62). Confirming our findings, we obtained the same result by immunofluorescence with three different specific antibodies to the three HP1 family members HP1, HP1ß, and HP1, with ectopically expressed GFP-tagged HP1, by ChIP analysis, and by immunoFISH. In addition, we showed that inhibition of DNA methylation by 5'-AzaC triggered the same relocalization, showing that the effect of the HDIs is due to the disruption of chromatin rather than another nonchromatin target of the HDIs, e,g., p53 (17, 67). Significantly, the previous studies examining the effects of HDIs on HP1 proteins at the pericentromeres were typically carried out after a much longer duration of HDI treatment and, most notably, typically in marsupial, murine, or transformed human cells. In fact, none of the previous reports showed raw data from primary human cells (8, 51, 62). Moreover, we, too, have found that the acute treatment of murine cells with TSA or chronic treatment of transformed human cells with TSA, replicating the conditions of a previous study (62), results in the loss of HP1 proteins from pericentromeres (see Fig. S3B and C in the supplemental material). In sum, the behavior of HP1 proteins after acute HDI treatment of primary human cells is profoundly different from results reported previously in other cell types with different treatment protocols.
Our data indicate that the recruitment of HP1 proteins to the pericentromeres depends on HIRA-mediated deposition of the histone variant, histone H3.3, into chromatin, seemingly by exchange with the canonical histone H3.1 subtype, since the abundance of the canonical histone in pericentromeric DNA decreases at the same time that the variant increases. Interestingly, newly synthesized histone H3 in human cells has been reported to be unacetylated (23, 61). Moreover, a recent study by Almouzni and coworkers has shown that a proportion of "free" non-chromatin-bound histone H3.3 is methylated to create H3K9Me2 (30). Thus, HP1 proteins might be recruited to pericentromeres by their binding to newly deposited histone H3.3 that is methylated on lysine 9 prior to its deposition or becomes methylated after its incorporation into chromatin. Since the abundance of H3K9Me2 and H3K9Me3 at the pericentromeres does not increase in HDI-treated cells, deposition of newly synthesized histone H3.3 may serve to maintain the preexisting level of H3K9Me in the face of rising histone acetylation, implying that more HP1 proteins bind to the same number of H3K9Me binding sites in HDI-treated cells. Conceivably, H3K9Me moieties are more accessible to HP1 in the context of hyperacetylated "open" chromatin (64). The idea that histone H3.3 recruits HP1 proteins appears to contradict several recent reports that link histone H3.3 to transcription activation (1, 34, 36, 57, 70). However, it should be noted that histone H3.3 per se has not been shown to cause or contribute to transcription activation. Moreover, a proportion of histone H3.3 does carry transcription modifications characteristic of silent chromatin, such as H3K9Me (14, 30, 34). Also, histone H3.3 accumulates in nondividing, differentiated cells and fibroblasts approaching senescence, in some cases to ca. 90% of the total histone H3, with presumably the majority being in inactive chromatin (5, 6, 13, 22, 44, 47, 52, 65, 71). Moreover, upon egg fertilization in flies and worms, the sperm chromatin is remodeled prior to DNA replication using histone variant H3.3, seemingly in a transcription-independent manner (28, 42). Therefore, an alternative view of histone H3.3 is that it is a replacement variant histone, associated with any "change in chromatin state," that is incorporated in a replication-independent manner during transcription, sperm chromatin remodeling or, as proposed here, as part of a dynamic response to rectify defects in chromatin modifications.
Many of the proteins now known to contribute to the cellular response to DNA damage, such as ATM, BRCA1, and the Fanconi's anemia gene products, were initially implicated in this process based on their dynamic relocalization in response to genotoxic stress (27, 33, 58) and/or the sensitivity of cells lacking these proteins to DNA-damaging agents (2, 69). In some respects, the response of HP1 proteins to CDAs is analogous to the response of these DNA repair proteins to DNA damage: HP1 proteins relocalize to sites of altered modifications in response to CDAs, and cells deficient in HP1 proteins are extremely sensitive to killing by CDAs. Thus, it is tempting to speculate that one function of HP1 proteins is to serve as dynamic responders to the perturbation of heterochromatin modifications, thereby rescuing heterochromatin function and protecting the cells from those perturbations. We note that HDIs occur naturally in the environment. For example, the concentration of butyrate in the colon can reach millimolar concentrations as a consequence of the bacterial fermentation of carbohydrate (56). Thus, one function of HP1 proteins might be to protect cells from the detrimental effects of such toxins.
Extending this view, HP1 proteins might also respond to alterations in chromatin structure caused by physiological nuclear processes. This might be why HP1 proteins are dynamically bound to chromatin, exhibiting surprisingly high off rates and on rates (7). This dynamic binding behavior would be expected to facilitate their recruitment to sites of altered chromatin. Also consistent with this idea, it was recently shown that HP1 is recruited to transcriptionally active genes during the elongation phase (66). HP1 might play a dynamic role in reestablishing transcriptionally silent chromatin after disruption of the chromatin structure by the passing RNA polymerase. Interestingly, previous reports have shown that the activation of gene expression by HDIs is a transient response, suggesting that cells are somehow able to suppress the transcription-activating effects of HDIs (45). Consistent with the idea that HP1 proteins rescue defects in chromatin structure and function outside of pericentromeres, a proportion of TSA-treated HP1ßN-expressing cells appeared to die during interphase (data not shown). Together, these results indicate that HP1 proteins might play a more general role in the dynamic rescue of chromatin defects than that described here.
In summary, we have shown that, in response to a variety of small molecules that perturb heterochromatin, HP1 proteins are dynamically relocalized to sites of altered heterochromatin at the pericentromeres. This relocalization is essential to maintain the HP1-binding protein hMis12 at the kinetochores and suppress lethal defects in mitosis. We propose that these results point to a new function of HP1 proteins as dynamic responders to the perturbation of chromatin modifications and as essential players in a chromatin "repair-like" process.
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ACKNOWLEDGMENTS |
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antibody, J. B. Rattner for the ACA antibody, Richard Katz for providing apicidin and valproic acid, Inma Ibanez and Paul Cairns for AzaC, Andy Godwin for human ovarian surface epithelial cells, and Kenneth Zaret for helpful comments. This study was supported by NIH grant GM062281 and LLS grant 1520-04 to P.D.A.; an AFAR grant to R.Z.; NIH grant GM49351 to J.P.; and NIH grants GM44762, CA99423, and CA75138 and core grant CA06927 to T.J.Y. and S.-T.L.
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FOOTNOTES |
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Published ahead of print on 13 November 2006.
Supplemental material for this article may be found at http://mcb.asm.org/.
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