Loss of HCF-1-Chromatin Association Precedes Temperature-Induced Growth Arrest of tsBN67 Cells

doi:10.1128/MCB.21.11.3820-3829.2001

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Molecular and Cellular Biology, June 2001, p. 3820-3829, Vol. 21, No. 11
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.11.3820-3829.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Loss of HCF-1-Chromatin Association Precedes Temperature-Induced Growth Arrest of tsBN67 Cells

Joanna Wysocka,¹ Patrick T. Reilly,¹^,² and Winship Herr¹^,^*

Cold Spring Harbor Laboratory, Cold Spring Harbor, New York 11724,¹ and Program in Molecular and Cellular Biology, State University of New York, Stony Brook, New York 11794²

Received 3 January 2001/Returned for modification 5 February 2001/Accepted 5 March 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Human HCF-1 is a large, highly conserved, and abundant nuclear protein that plays an important but unknown role in cell proliferation.It also plays a role in activation of herpes simplex virus immediate-earlygene transcription by the viral regulatory protein VP16. A singleproline-to-serine substitution in the HCF-1 VP16 interaction domaincauses a temperature-induced arrest of cell proliferation in hamstertsBN67 cells and prevents transcriptional activation by VP16.We show here that HCF-1 is naturally bound to chromatin in uninfectedcells through its VP16 interaction domain. HCF-1 is chromatinbound in tsBN67 cells at permissive temperature but dissociatesfrom chromatin before tsBN67 cells stop proliferating at the nonpermissivetemperature, suggesting that loss of HCF-1 chromatin associationis the primary cause of the temperature-induced tsBN67 cell proliferationarrest. We propose that the role of HCF-1 in cell proliferationis to regulate gene transcription by associating with a multiplicityof DNA-bound transcription factors through its VP16 interactiondomain.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Regulated cell proliferation requires the coordination of many distinct cellular processes. Much of this coordination occursthrough the regulation of gene expression, often at the levelof transcription. Consequently, transcriptional regulation isoften altered when cells become oncogenic and manipulated by virusesto promote infection. For example, the DNA-bound transcriptionalactivator E2F and the E2F-associated retinoblastoma (Rb) transcriptionalrepressor protein are important players in the control of cellproliferation and their activities are often disrupted duringoncogenesis and manipulated by viral regulatory proteins duringDNA tumor virus infection (see references 4 and 22 for reviews).Other less well-understood regulators of cell proliferation includethe cellular protein HCF-1. HCF-1 is a highly conserved and abundantnuclear protein that plays a known role in herpes simplex virustype 1 (HSV-1) infection (for reviews, see references 10 and23) and an important but unknown role in cell proliferation(7).

Many aspects of HCF-1 make it an unusual protein. It is initially synthesized as a large precursor molecule of over 2,000amino acids (29). After synthesis, HCF-1 migrates to the nucleus,where it is cleaved repeatedly at a series of six 26-amino-acidrepeats located near the middle of the protein (11, 29, 30).These cleavages result in a heterogeneous collection of stableamino (HCF-1_N)- and carboxy (HCF-1_C)-terminal subunits that remainnoncovalently associated (30). Although the unusual maturationprocess of HCF-1 has been well documented, how HCF-1 functionsnormally in the cell is essentiallyunknown.

Much more is known about the role of HCF-1 during HSV-1 infection. When HSV-1 first infects a cell, HCF-1 forms a stable heterodimericcomplex with the viral transcriptional regulator VP16 (also knownas Vmw65 and $alpha$ -TIF), which is delivered by the infecting virion.Together, the HCF-1-VP16 complex binds to the cellular transcriptionfactor Oct-1 on DNA to form a multiprotein transcriptional activatorcomplex $---$ the VP16-induced complex $---$ on VP16-responsive elements foundin HSV-1 immediate-early promoters (for reviews, see references10 and 23). Although HCF-1 is a large protein, only the 380amino-terminal residues of HCF-1 are necessary to associate withVP16 and promote VP16-induced complex formation (13, 28).These 380 amino acids contain six tandem repeats called HCF-1_Kelrepeats because they are related to repeats found in the Drosophilaprotein Kelch (31); these repeats probably form a stable structurecalled a $beta$ propeller (3, 28) and are collectively referredto, interchangeably, as the Kelch or VP16 interactiondomain.

HCF-1 is known to be involved in cell proliferation because a single proline-to-serine missense mutation at position 134 inthe VP16 interaction domain (P134S) causes temperature-inducedcell proliferation arrest in the hamster cell line tsBN67 (7).tsBN67 cells proliferate normally at the permissive temperatureof 33.5°C, but a few cell divisions after transfer to the nonpermissivetemperature of 40°C, these cells enter a stable cell proliferationarrest. HCF-1 processing and stability are nearly normal in tsBN67cells at the nonpermissive temperature, but association with VP16is disabled, suggesting that the arrest phenotype is caused byloss of HCF-1 association with a cellular protein(s) mimickedby VP16 (7, 28). Although sufficient for formation of theVP16-induced complex, however, the HCF-1 VP16 interaction domainis not sufficient to rescue the tsBN67 cell proliferation defect;a neighboring basic region within the HCF-1_N subunit is also requiredfor rescue (28).

Although little is known of how HCF-1 promotes cell proliferation, multiple molecular targets of HCF-1 function have beeninferred from the results of Saccharomyces cerevisiae two-hybridand in vitro protein-binding assays. The basic leucine zipperproteins LZIP (also known as Luman) and Zhangfei (ZF) associatewith the HCF-1 VP16 interaction domain in a manner similar tothat of VP16 (5, 15-17); all three proteins possess a shorttetrapeptide HCF-1-binding motif $---$ (D/E)HXY (where X denotes avariable position) $---$ and their association with HCF-1 is sensitiveto the tsBN67 point mutation. Two transcription factors associatewith the HCF-1 basic region: GABP (26) and Sp1 (8). Last,the HCF-1_C subunit can associate with protein phosphatase 1 (1).Although these protein association studies (1, 5, 8, 15-17, 26)suggest that HCF-1 plays a role in transcriptional regulation,possibly through modulation of protein phosphorylation, a naturalmolecular function of HCF-1 remains to beelucidated.

We show here that, in uninfected cells, HCF-1 is associated with chromatin through its VP16 interaction domain. In tsBN67cells, HCF-1 dissociates from chromatin preceding temperature-inducedcell proliferation arrest. These results suggest that HCF-1 playsan active role in cell proliferation through the regulation ofchromosomal geneexpression.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Small-scale biochemical fractionation. Small-scale biochemical fractionation was performed as described previously (20). Briefly, 1 × 10⁷ to 2 × 10⁷ cells were collected, washed with phosphate-buffered saline (PBS),and resuspended at 4 × 10⁷ cells/ml in buffer A (10 mM HEPES [pH 7.9], 10 mM KCl, 1.5 mMMgCl₂, 0.34 M sucrose, 10% glycerol, 1 mM dithiothreitol, andprotease inhibitor cocktail [Boehringer]). Triton X-100 was added(0.1% final concentration), the cells were incubated on ice for8 min, and nuclei (fraction P1) were collected by centrifugation(5 min, 1,300 × g, 4°C). The supernatant (fraction S1) was clarifiedby high-speed centrifugation (5 min, 20,000 × g, 4°C), and thesupernatant (fraction S2) was collected. The P1 nuclei were washedonce in buffer A and lysed for 30 min in buffer B (3 mM EDTA,0.2 mM EGTA, 1 mM dithiothreitol, and protease inhibitor cocktail[Boehringer]), and insoluble chromatin (fraction P3) and soluble(fraction S3) fractions were separated by centrifugation (5 min,1,700 × g, 4°C). The P3 fraction was washed once with buffer Band resuspended either in sodium dodecyl sulfate (SDS)-Laemmlibuffer (and boiled for 10 min) or in nuclease digestionbuffer.

MNase treatment. For micrococcal nuclease (MNase) treatment, the P3 pellet was resuspended in a solution containing 10 mM Tris, 10 mM KCl,and 1 mM CaCl₂ and 1 U of MNase (Sigma) was added. After 37°Cincubations for the times indicated in Fig. 1C, the reaction wasstopped with EGTA (1 mM final concentration). Soluble and insolublecomponents were then separated by centrifugation (5 min, 1,700× g, 4°C). The pellet was resuspended in SDS-Laemmli buffer andboiled for 10 min. Half of the supernatant was used for immunoblotanalysis, the remainder was extracted with phenol-chloroform andethanol precipitated, and its DNA content was analyzed by agarosegelelectrophoresis.

Retroviral vectors and stable HCF-1 synthesis. A pBabeFLAG retroviral expression vector was constructed by inserting oligonucleotides encoding the FLAG epitope tag (DYKDDDDK)into the pBabe-Puro vector (21). XbaI-BamHI cDNA fragments encodingeither the wild-type human HCF-1_N1011 subunit (HCF-1 residues2 to 1011), its alternative splice variant HCF-1_N1011382-450,its tsBN67 mutant version HCF-1_N1011/P134S, or the VP16 interactiondomain (HCF-1_N380) alone were inserted into the pBabeFLAG vector.Populations of cells stably synthesizing FLAG-tagged forms ofHCF-1 were obtained by retroviral gene transfer with the Phoenixamphotropic virus packaging line as described previously (25).Infected HeLa and IMR90 cells were selected by culturing cellsin 10% fetal bovine serum (FBS) in Dulbecco's modified Eagle'smedium (DMEM) containing 2 µg of puromycin per ml for 7 to 10days. Subpopulations of infected cells were frozen for futureuse, and others were lysed and tested for recombinant HCF-1 synthesisby FLAG tag immunoblot analysis. Cells infected with the pBabeFLAGparent vector were used ascontrols.

Immunoblot analysis. Polyclonal HCF-1_N subunit ( $alpha$ N18 [7]) and HCF-1_c subunit ( $alpha$ H12 [29]) antisera have been described previously. They arereferred to here as $alpha$ HCF-1_N and $alpha$ HCF-1_C, respectively, and wereused at a 1:3,000 dilution for immunoblot probing. Anti-FLAG (M2;Sigma) and anti-MEK2 (M24520; Transduction Laboratories) antiserawere obtained commercially. ORC2 and MCM3 antisera were kind giftsof J. Méndez and B. Stillman (Cold Spring Harbor Laboratory).Immunoblots were prepared by semidry transfer and developed bychemiluminescence (SuperSignal;Pierce).

Immunofluorescence. IMR90 cells were seeded onto sterile coverslips. After 24 h, cells were (i) washed with PBS, (ii) fixed for 20 min with 4%paraformaldehyde, (iii) permeabilized for 5 min with 0.1% TritonX-100 in PBS, (iv) washed twice with PBS, and (v) blocked for20 min with 5% bovine serum albumin in PBS. After being rinsedwith PBS, coverslips were incubated for 1 h with protein A-purified $alpha$ HCF-1_N antibody and excess specific (N18) or nonspecific (FLAG)peptide. The samples were then washed five times with PBS andincubated for 1 h with Texas Red-conjugated secondary antibody.After being extensively washed with PBS, the coverslips were stainedwith DAPI (4',6'-diamidino-2-phenylindole) and mounted, and fluorescencewas observed with a Zeiss fluorescencemicroscope.

HCF-1 quantitation. A six-His tag-HCF-1_N380 fusion protein was synthesized to high levels in Escherichia coli and prepared by bacterial lysiswith SDS-Laemmli buffer. The levels of six-His tag-HCF-1_N380 fusionprotein in the lysate were determined by SDS-polyacrylamide gelelectrophoresis and Coomasie staining of a twofold serial dilutionof the lysate alongside a serial dilution of bovine serum albuminof known concentration. HeLa or IMR90 cells were counted and directlylysed in SDS-Laemmli buffer. The levels of HCF-1 were directlycompared to those of the six-His tag-HCF-1_N380 fusion proteinby parallel immunoblot analysis with the $alpha$ HCF-1_Nantiserum.

BHK21 and tsBN67 cells. BHK21 and original tsBN67 cells were a kind gift of T. Nishimoto (Kyushu University). The tsBN67 cells were single-cell subclonedto produce the tsBN67_HR1 line used here. tsBN67_HR1 cells displaythe same temperature-sensitive proliferation defect as the originaltsBN67 cells. Cells were grown in DMEM supplemented with 10% FBS.To measure tsBN67_HR1 cell proliferation arrest at 40°C, 2 × 10⁴ BHK21 or tsBN67_HR1 cells were (i) seeded onto 6-cm-diameter plates,(ii) maintained at 33.5°C for 48 h, and (iii) transferred to 40°C,and portions were collected every 12 h by trypsinization and countedwith a hemacytometer. To arrest tsBN67 cell proliferation by limitingserum, asynchronous populations of tsBN67_HR1 cells were incubatedat 33.5°C for 24 h in DMEM containing 0.25% FBS and subsequentlytransferred to 40°C and harvested at the times indicated in Fig.7.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

HCF-1 associates with chromatin. HCF-1 is a nuclear protein and, as part of the HSV-1 VP16-induced complex, associates with DNA. We therefore asked whether,in uninfected cells, HCF-1 is associated with DNA in the formof chromatin. We used a small-scale biochemical fractionationscheme (20) illustrated in Fig. 1A. HeLa cell lysates preparedwith a nonionic detergent were divided by sequential centrifugationinto three fractions: (i) a fraction largely consisting of solublecytosolic components called S2, (ii) a fraction containing solublenuclear components called S3, and (iii) an insoluble pellet fractioncontaining chromatin and nuclear matrix components called P3.The S2 fraction probably also contains soluble nuclear componentsowing to permeabilization of the nuclear membrane by the nonionicdetergent.

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FIG. 1. HCF-1 is chromatin associated. (A) Biochemical fractionation scheme (see Materials and Methods for details). Final fractions used for analysis $---$ S2, S3, and P3 $---$ are boxed. (B) HCF-1 is enriched in the chromatin-containing P3 fraction. HeLa cells were subjected to biochemical fractionation, and cell-equivalent amounts of fractions S2, S3, and P3 were probed by immunoblotting with $alpha$ HCF-1_N (upper left panel), $alpha$ HCF-1_C (upper right panel), $alpha$ ORC2 (lower left panel), and $alpha$ MEK2 (lower right panel) antisera. The positions of the heterogeneous HCF-1 subunits are indicated by double dots. (C) HCF-1 can be solubilized in the chromatin-enriched P3 fraction by treatment with MNase. The P3 fraction was resuspended in nuclease buffer and treated with MNase (see Materials and Methods) for the times indicated. The digested suspension was then centrifuged, and the supernatant (upper panel) and pellet (lower panel) were collected and analyzed by immunoblotting with $alpha$ HCF-1_N (lanes 1 to 4) and $alpha$ MCM3 (lanes 5 to 8) antisera.

To verify appropriate fractionation by this procedure, we probed the three different fractions by immunoblot analysis forthe chromatin-associated DNA replication factor ORC2 and the cytoplasmicsignal transduction kinase MEK2. As shown in Fig. 1B (lower panels),consistent with the desired fractionation, the majority of theORC2 protein was in the P3 chromatin-containing pellet (comparelanes 1 to 3) whereas the MEK2 protein was in the S2 cytosolicfraction (compare lanes 4 to6).

Using the same fractions, we analyzed the distribution of the native HCF-1_N and HCF-1_C subunits with HCF-1_N and HCF-1_C subunit-specificantisera. The large majority of the heterogeneous collection ofendogenous HCF-1_N (lanes 1 to 3) and HCF-1_C (lanes 4 to 6) subunitswere recovered in the P3 chromatin-containing pellet (Fig. 1B,upper panels). Similar results were obtained with human IMR90and 293 cells (see below and data not shown). These results suggestthat HCF-1 subunits are attached to chromatin or some other insolublestructure in thenucleus.

To distinguish between these two possibilities, we treated the P3 fraction with MNase to solubilize the chromatin. As shownin Fig. 1C, the majority of the HCF-1 in the P3 fraction becomessoluble within 2 to 5 min of MNase treatment (lanes 1 to 4, comparethe pellet and supernatant panels). This pattern of HCF-1 MNasesolubilization parallels that of the chromatin-bound DNA replicationprotein MCM3 (lanes 5 to 8). Analysis of the DNA in the MNase-treatedsamples showed that DNA release from the P3 pellet paralleledHCF-1 solubilization (data not shown). These results indicatethat HCF-1 is associated with nuclease-sensitive chromatin inproliferating tissue culturecells.

The HCF-1_C subunit is dispensable for chromatin association by the HCF-1_N subunit. To map the regions of HCF-1 responsible for directing it to chromatin, we used a retroviral expression vector to direct synthesisof four epitope-tagged truncations of HCF-1 in HeLa cells. Figure2A shows the overall structure of HCF-1 with the positions of(i) defined structural regions (e.g., HCF-1_Kel repeats and basicregion), (ii) functional regions (e.g., VP16-induced complex formationand HCF-1 subunit association), and (iii) regions involved inassociation with heterologous viral (VP16) and cellular (e.g.,LZIP, GABP, and PP1) proteins. Figure 2B shows the series of fourFLAG epitope-tagged HCF-1 proteins used to study HCF-1 recruitmentto chromatin. Each of these epitope-tagged proteins is a derivativeof the HCF-1_N subunit: (i) HCF-1_N1011 represents the wild-typeHCF-1_N subunit, (ii) HCF-1_N1011382-450 represents theproduct of an alternative HCF-1 pre-mRNA splice which does toassociate with HCF-1_C subunits (30), (iii) HCF-1_N1011/P134Scarries the tsBN67 P134S mutation, and (iv) HCF-1_N380 representsthe VP16 interaction domain alone.

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FIG. 2. The HCF-1 VP16 interaction domain is both necessary and sufficient for chromatin association. (A) Overall structure of HCF-1. Above and below a diagram of HCF-1 are shown the positions of (i) regions involved in association with the proteins indicated (top), (ii) structural or sequence elements (immediately above the diagram), and (iii) functional regions (below the diagram). Within the diagram, structural and functional features of HCF-1 are indicated from left to right as follows: the VP16 interaction or Kelch domain (gray box), the HCF-1_C subunit association element (stippled box), the region deleted by the alternative pre-mRNA splice lacking residues 382 to 450 (triangle), the basic region (hatched box), the functional (filled triangles) and nonfunctional (open triangles) HCF-1_PRO processing repeats, the acidic region (black box), the HCF-1_N subunit association element with fibronectin type 3 repeats (stippled box with arrowheads), and the carboxy-terminal NLS (black box). VIC, VP16-induced complex. (B) Schematic of four FLAG epitope-tagged carboxy-terminal HCF-1 truncations used in this study. (C) Stable populations of HeLa cells synthesizing either FLAG-tagged HCF-1_N1011 (lanes 4 to 6), HCF-1_N1011382-450 (lanes 7 to 9), HCF-1_N1011/P134S (lanes 10 to 12), or no recombinant HCF-1 protein (lanes 1 to 3) were subjected to biochemical fractionation as described in the legend to Fig. 1A. S2 (lanes 1, 4, 7, and 10), S3 (lanes 2, 5, 8, and 11), and P3 (lanes 3, 6, 9, and 12) fractions were analyzed by immunoblotting with $alpha$ FLAG (upper panel) and $alpha$ HCF-1_N (lower panel) antisera. The positions of endogenous HCF-1_N subunits are indicated by the double dots, the positions of FLAG-tagged recombinant HCF-1_N proteins are indicated by the arrowheads, and the position of an $alpha$ FLAG antiserum-cross-reacting species is indicated by the asterisks. WT, wild type. (D) Stable populations of HeLa cells synthesizing FLAG-tagged HCF-1_N380 (lanes 4 to 6) or no recombinant HCF-1 protein (lanes 1 to 3) were subjected to biochemical fractionation and probed with the $alpha$ FLAG antiserum as described for part C. The position of the HCF-1_N380 fragment is indicated by the arrowhead.

Figure 2C shows the results of biochemical fractionation of cells with each FLAG-tagged HCF-1_N1011 derivative. The recombinantproteins were visualized alone with the $alpha$ FLAG-tag antiserum (upperpanel) or together with the endogenous proteins with the $alpha$ HCF-1_Nsubunit antiserum (lower panel). The $alpha$ FLAG-tag analysis showsthat the HCF-1_N1011 protein is recovered in the P3 fraction (lanes4 to 6, upper panels); this HCF-1_N1011 protein could be solubilizedby MNase treatment (data not shown), indicating that it is chromatinbound. The HCF-1_N1011382-450 protein, which does notassociate with the HCF-1_C subunit (30), is also present in thechromatin-containing P3 fraction (compare lanes 7 to 9, upperpanel), indicating that association with the HCF-1_C subunit isdispensable for chromatin association by the HCF-1_Nsubunit.

Probing with the $alpha$ HCF-1_N antiserum (Fig. 2C, lower gels) shows that the recombinant HCF-1_N proteins are synthesized at levelssimilar to those of the endogenous proteins and that the endogenousHCF-1_N subunits are still largely associated with chromatin (comparelanes 1 to 12). Thus, in these cells the endogenous HCF-1_N proteinsare not dislodged from the chromatin to any greatextent.

The HCF-1 VP16 interaction domain is necessary and sufficient for chromatin association. The HCF-1_N subunit contains two functional regions that might be involved in chromatin association: the VP16 interaction domainand the basic region. Both of these regions are required to rescuethe tsBN67 HCF-1 cell proliferation defect (28) and can associatewith cellular DNA-binding proteins (5, 8, 16, 26). Todetermine whether the VP16 interaction domain is required forHCF-1_N-chromatin association, we tested whether the HCF-1_N1011/P134Sprotein, which fails to associate with VP16 (28), LZIP (5),and ZF (15), associates with chromatin. Indeed, the HCF-1_N1011/P134Ssubunit failed to associate with chromatin (Fig. 2C, lanes 10and 12, upper panel) and did not cofractionate with the endogenousHCF-1_N subunits (compare lanes 10 and 12, lower panel). Thus,an HCF-1 point mutation, which is known to prevent HCF-1 associationwith proteins that bind DNA, also prevents HCF-1_N associationwith chromatin. Together with the lack of any evidence that HCF-1normally binds DNA directly, these results suggest that HCF-1is tethered to DNA by interaction with a protein receptor at leastin part through its VP16 interaction domain. Because in this experimentthe HCF-1_N1011/P134S mutant protein is present alongside the chromatin-boundwild-type endogenous protein, the lack of chromatin-bound HCF-1_N1011/P134Sprotein suggests that HCF-1_N subunits do not recruit each otherto chromatin through higher-order homomeric complexformation.

To test whether the HCF-1 VP16 interaction domain is not only necessary but also sufficient for HCF-1_N-chromatin association,we asked whether the HCF-1_N380 fragment (Fig. 2B) can associatewith chromatin. The HCF-1_N380 fragment is indeed largely presentin the P3 fraction (compare lanes 4 to 6). Thus, the VP16 interactiondomain is both necessary and sufficient for HCF-1_N-chromatin association.These results suggest that HCF-1_N subunits are tethered to DNAin chromatin through their VP16 interaction domains and that thebasic region is dispensable for HCF-1-chromatinassociation.

Nuclear localization of HCF-1_N1011 but not the HCF-1_N1011/P134S mutant. Given the results of previous studies of HCF-1 subcellular localization (12, 27), HCF-1_N subunit-chromatin associationis paradoxical. The previous studies have shown that HCF-1 nuclearlocalization is directed by a single nuclear localization signal(NLS) located at the carboxy terminus of HCF-1 (Fig. 2A). Whenit is synthesized independently of the HCF-1_C subunit by transientoverexpression, the HCF-1_N subunit remains in the cytoplasm (12,27). How then is the HCF-1_N subunit present in the chromatin-containingP3 fraction after stable synthesis in HeLa cells? We hypothesizedthat, if not synthesized at very high levels as during transientoverexpression, the majority of the HCF-1_N subunits may be broughtto chromatin and hence the nucleus by the VP16 interactiondomain.

To test this hypothesis, we assayed HCF-1_N1011 and HCF-1_N1011/P134S localization by immunofluorescence in IMR90 cells carryingthe FLAG tag retroviral expression vectors as shown in Fig. 3.We chose IMR90 cells because the suspension HeLa cells used forrecombinant HCF-1 synthesis are less amenable to immunofluorescenceanalysis. As in HeLa cells, in these IMR90 cells, the wild-typeHCF-1_N1011 (Fig. 3A, lanes 4 to 6), but not the HCF-1_N1011/P134Sfragment (lanes 7 to 9), is associated with the chromatin-containingP3 fraction.

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FIG. 3. Nuclear localization of the HCF-1_N1011 but not the HCF-1_N1011/P134S polypeptide. (A) Stable populations of IMR90 cells synthesizing either FLAG-tagged HCF-1_N1011 (lanes 4 to 6), HCF-1_N1011/P134S (lanes 7 to 9), or no recombinant HCF-1 protein (lanes 1 to 3) were subjected to biochemical fractionation as described for Fig. 1A. S2 (lanes 1, 4, and 7), S3 (lanes 2, 5, and 8), and P3 (lanes 3, 6, and 9) fractions were analyzed by immunoblotting with $alpha$ FLAG antiserum. (B) The same IMR90 cell populations synthesizing FLAG-tagged HCF-1_N1011 (b, e, and h), HCF-1_N1011/P134S (c, f, and i), or no recombinant HCF-1 protein (a, d, and g) were subjected to immunofluorescence analysis with purified $alpha$ HCF-1_N antibodies in the presence of the peptide (N18) used to raise the antiserum (g to i) or of a nonspecific peptide (FLAG) (d to f). The nuclei in the cells shown in images d to f were identified by staining with DAPI (a to c). WT, wild type.

For the immunofluorescence analysis, the $alpha$ FLAG antiserum was not sufficiently sensitive to detect the recombinant HCF-1_N proteins.We therefore used the $alpha$ HCF-1_N antiserum to detect both endogenousand recombinant HCF-1_N proteins in control IMR90 cells (Fig. 3B,panels a, d, and g) or IMR90 cells synthesizing wild-type (b,e, and h) or P134S mutant (c, f, and i) HCF-1_N1011 protein. Thecells were stained with DAPI to identify nuclei (Fig. 3B, panelsa to c) and with the $alpha$ HCF-1_N antipeptide serum in the absence(d to f) or presence (g to i) of specific peptide to establishthe specificity of the HCF-1_N staining; indeed, the $alpha$ HCF-1_N antiserumproduces a low level of nonspecific staining (g to i). The controlcells (Fig. 3B, panel d) exhibit the typical predominantly nuclearimmunofluorescence pattern of endogenous HCF-1 (11). When thewild-type recombinant HCF-1_N1011 subunit is present in the IMR90cells, there is an increase in nuclear staining (compare Fig.3B, panels d and e), whereas when the mutant HCF-1_N1011/P134Ssubunit is present, there is an increase in cytoplasmic staining(compare Fig. 3B, panels d and f). These results are consistentwith nuclear localization of the wild-type but not the P134S mutantHCF-1_N1011 subunit and suggest that the predominantly cytoplasmiclocalization of the wild-type HCF-1_N subunit observed previouslyduring transient overexpression results from the very high levelsof transient HCF-1_N subunit synthesis. Perhaps an HCF-1_N receptorprotein(s) can bring the HCF-1_N subunit to the nucleus and chromatinand this receptor is saturated by HCF-1_Noverexpression.

HCF-1 is an abundant protein. The experiments described above suggest that HCF-1 is targeted to chromatin through protein-protein association. Purificationof HCF-1 in a previous study has suggested that it is an abundantprotein (29), but the number of molecules in a cell is unknown.Such a number would indicate how many chromatin-bound receptorproteins are required to recruit the HCF-1_N subunit to chromatinif they associate stoichiometrically as in the VP16-induced complex.To determine the number of HCF-1 molecules in a cell, we comparedthe immunoblot signal of endogenous HCF-1 from a known numberof cells to that of a known concentration of HCF-1_N380 proteinsynthesized in E. coli (see Materials and Methods). From the comparison,whose results are shown in Fig. 4, we obtained a minimal estimateof the number of HCF-1 molecules per cell by estimating that 10⁵ cells (lane 2, lower panel) contain 80 fmol of protein (lane3, upper panel) or about 5 × 10⁵ HCF-1 molecules per HeLa cell. We estimated about half that amountper IMR90 cell (data not shown). Thus, even if our number is notabsolutely precise, HCF-1 is an abundant protein probably presentat more than 100,000 molecules per HeLa or IMR90 cell. This resultsuggests that, if only one or a few proteins target HCF-1 to chromatin,one or more of them should be very abundant. Alternatively, alarge number of less abundant proteins may target HCF-1 to chromatin.

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FIG. 4. HeLa cells contain over 100,000 molecules of HCF-1 per cell. The immunoblot signal of a twofold titration of bacterially synthesized HCF-1_N380 protein of known molar concentration (upper panel; the number of femtomoles of HCF-1_N380 protein in each lane is indicated) is directly compared to the immunoblot signal of a twofold titration of HCF-1 from a known number of HeLa cells (lower panel; the number of cells used for each lane is indicated).

HCF-1 chromatin association is temperature sensitive in tsBN67 cells. The tsBN67 P134S mutation prevents chromatin association of HCF-1_N subunits in HeLa cells grown at 37°C (Fig. 2C). The samemutation causes temperature-sensitive proliferation arrest intsBN67 cells at 40°C. To determine whether there is a relationshipbetween HCF-1 chromatin association and the temperature-sensitivedefect in tsBN67 cell proliferation, we performed biochemicalfractionation on four sets of cells: BHK21 and tsBN67 cells grownat permissive (33.5°C) and nonpermissive (40°C) temperatures for64h.

To monitor the fractionation of the tsBN67 cell extracts, the distribution of chromatin-bound ORC2 and cytosolic MEK2 in thedifferent fractions was assayed as shown in Fig. 5C and D. Inboth cell lines and at both temperatures, ORC2 was present exclusivelyin the P3 chromatin pellet (Fig. 5C, lanes 1 to 12), indicatingthat the soluble fractions were not contaminated with chromatin-associatedproteins, and MEK2 was solely recovered in the cytosolic fractionS2 (Fig. 5D, lanes 1 to 12), indicating that the extraction ofcytosolic proteins was complete.

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FIG. 5. The HCF-1-chromatin association is temperature sensitive in tsBN67 cells. BHK21 (lanes 1 to 3 and 7 to 9) and tsBN67_HR1 (lanes 4 to 6 and 10 to 12) cells grown at 33.5°C (lanes 1 to 6) or 40°C (lanes 7 to 12) for 64 h were biochemically fractionated as described for Fig. 1A, and the resulting S2 (lanes 1, 4, 7, and 10), S3 (lanes 2, 5, 8, and 11), and P3 (lanes 3, 6, 9, and 12) fractions were analyzed by immunoblotting with $alpha$ HCF-1_N (A), $alpha$ HCF-1_C (B), $alpha$ ORC2 (C), and $alpha$ MEK2 (D) antisera. The protein contents of separate fractionations were normalized by Bradford assay of each S2 fraction. The positions of the relevant polypeptides are indicated.

In the same extracts, the HCF-1_N and HCF-1_C subunits behaved similarly in this assay. At 33.5°C, most, albeit (unlike withHeLa, 293, and IMR90 cells grown at 37°C) not all, of the wild-typeHCF-1 in BHK21 cells was chromatin associated (Fig. 5A and B,lanes 1 to 3). In tsBN67 cells grown at 33.5°C, about half ofthe HCF-1 was chromatin bound (Fig. 5A and B, lanes 4 to 6). Thus,in contrast to the recombinant HCF-1_N1011/P134S protein in HeLacells grown at 37°C, the P134S mutant HCF 1 protein can bind chromatinin tsBN67 cells grown at 33.5°C. At 40°C, however, whereas theHCF-1 from BHK21 cells was still predominantly chromatin bound(lanes 7 to 9), the HCF-1_N and HCF-1_C subunits from tsBN67 cellswere largely absent from the chromatin-containing P3 fraction(lanes 10 to 12). Although still probably being nuclear owingto the HCF-1_C NLS, the tsBN67 HCF-1 subunits were recovered insteadin the soluble S2 fraction, probably because soluble nuclear proteinsleak out of the nucleus during the fractionation procedure. Whateverthe reason, however, these results indicate that there is a correlationbetween HCF-1-chromatin association and tsBN67 cell proliferation.Furthermore, the lack of HCF-1_C subunit association with chromatinin temperature-arrested tsBN67 cells indicates that the associationof HCF-1_C subunits with chromatin is dependent on the VP16 interactiondomain of the HCF-1_Nsubunit.

Dissociation of tsBN67 HCF-1 from chromatin at 40°C is not immediate but precedes cell proliferation arrest. A characteristic property of tsBN67 cells is that they cease to proliferate at the nonpermissive temperature of 40°C aftera lag of a few cell divisions (7). To characterize the dissociationof HCF-1 from chromatin in tsBN67 cells at 40°C, we asked howthe timing of HCF-1-chromatin dissociation correlates with thetiming of the tsBN67 cell proliferation arrest. As shown in Fig.6A, as with the original tsBN67 cells (7), the subclone oftsBN67 cells used in this study (called tsBN67_HR1, see Materialsand Methods) stopped proliferating only after a lag of 36 to 48h at 40°C. In contrast, BHK21 cells continued to proliferate at40°C. Remarkably, biochemical fractionation of tsBN67 cells harvestedat different time points after the shift to 40°C revealed thatthe P134S mutant HCF-1 subunits were still bound to chromatinafter 4 h (Fig. 6B, compare lanes 2, 4, and 6) but began to dissociatemarkedly from chromatin by 8 h (lane 8) and were largely dissociatedfrom chromatin by 16 h (lane 10). More refined time points haveindicated that complete HCF-1_N-chromatin dissociation occurs afterabout 12 to 18 h at 40°C (data not shown). In contrast, in BHK21cells, HCF-1 was present in the chromatin-containing P3 fractionthroughout the course of the experiment (lanes 14, 16, and 18).Thus, in tsBN67 cells grown at 40°C, temperature-sensitive HCF-1dissociates from chromatin in the middle of the 36- to 48-h lagin cell proliferation arrest, preceding the arrest by about 20to 30 h.

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FIG. 6. Dissociation of HCF-1 from chromatin precedes tsBN67 cell proliferation arrest. (A) tsBN67_HR1 cells possess temperature-induced growth arrest characteristics similar to those of parental tsBN67 cells. BHK21 and tsBN67_HR1 cells were shifted to 40°C at 0 h, harvested, and counted at the indicated time points as described in Materials and Methods. N₀, number of cells at time of transfer to 40°C; N_t, number of cells at time of harvest. Each point is the average of results from two samples, with the deviation shown. (B) Timing of tsBN67 HCF-1_P134S dissociation from chromatin at 40°C. BHK21 (lanes 13 to 18) and tsBN67_HR1 (lanes 1 to 12) cells were grown at 40°C for the indicated times and subsequently harvested and fractionated as described for Fig. 1A. The resulting S2 (odd-numbered lanes) and P3 (even-numbered lanes) fractions were analyzed by immunoblotting with the $alpha$ HCF-1_N antiserum. The positions of the HCF-1_N polypeptides are indicated.

Arrest of tsBN67 cell proliferation before transfer to 40°C prevents temperature-induced dissociation of HCF-1 from chromatin. The aforementioned results indicate that HCF-1 dissociates from chromatin in tsBN67 cells at 40°C but only after a delay ofup to 18 h. We hypothesize two mechanisms for this delay: (i)a proliferation-independent mechanism in which it may simply taketime for the elevated temperature to dissociate the temperature-sensitiveHCF-1 from chromatin or (ii) a proliferation-dependent mechanismin which proliferation at 40°C is required to dissociate the mutantHCF-1 from chromatin. To discriminate between these two mechanisms,we starved tsBN67 cells of serum at 33.5°C for 24 h to arrestcell proliferation and then transferred the arrested cells to40°C, maintaining the low concentration of serum, and harvestedthem for biochemical fractionation at different time points forup to 30 h. At the time of transfer to 40°C, DNA content analysisshowed that the serum-starved tsBN67 cells were arrested witha G₁/G₀ DNA content (data not shown). As shown in Fig. 7 (upperpanels), the temperature-sensitive HCF-1 did not dissociate fromchromatin in serum-starved cells throughout the 30-h time course.In contrast, as expected, with an asynchronously proliferatingpopulation, HCF-1 was not detectable in the P3 chromatin-containingfraction by 18 h postshifting to 40°C (Fig. 7, lower panel). Thisanalysis provides two conclusions. First, because HCF-1 is boundto chromatin in the cells arrested by serum starvation (Fig. 7,upper panel), HCF-1 can be chromatin bound in nonproliferatingcells. Second, dissociation of the mutant HCF-1 from chromatinafter transfer to the nonpermissive temperature is proliferationdependent, suggesting that HCF-1 dissociation from chromatin isan active process during the course of tsBN67 cell proliferation.

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FIG. 7. tsBN67 HCF-1_P134S-chromatin association is stable at the nonpermissive temperature if tsBN67 cells are arrested before transfer to the nonpermissive temperature. tsBN67_HR1 cells were arrested by growth in 0.25% serum at 33.5°C for 24 h, and the arrested cells were subsequently transferred and maintained at 40°C in 0.25% serum (upper panels). In parallel, asynchronous tsBN67_HR1 cells maintained in 10% serum were analyzed (lower panels). Cells were harvested at the indicated times after transfer to 40°C and subjected to biochemical fractionation as described for Fig. 1A. The resulting S2 (odd-numbered lanes) and P3 (even-numbered lanes) fractions were analyzed by immunoblotting with the $alpha$ HCF-1_N antiserum. The positions of the HCF-1_N subunits are indicated by the dots; extra uncharacterized bands in the serum-starved samples are indicated by asterisks.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The study presented here clarifies our understanding of HCF-1 structure and function. They show that HCF-1 $---$ an abundant protein $---$ isbrought to DNA, probably indirectly, through a single structuralelement $---$ its VP16 interaction domain $---$ which is implicated solelyin protein-protein and not protein-DNAinteractions.

That the same region of HCF-1 is involved in both VP16-induced complex assembly and chromatin association suggests that theVP16-induced complex represents a model for how HCF-1 binds tochromatin naturally. Consistent with this hypothesis, VP16 andthe two cellular proteins that have been shown to associate withthe HCF-1 VP16 interaction domain share the tetrapeptide motif(D/E)HXY for HCF-1 binding, and in each case the P134S tsBN67mutation prevents protein association (5, 15, 17). By analogyto the VP16-induced complex, Fig. 8A illustrates how we believeHCF-1 associates with chromatin. We hypothesize that the HCF-1VP16 interaction (or Kelch) domain brings HCF-1 to the DNA bycontacting a solitary DNA-bound protein, such as LZIP, or a memberof a complex of DNA-bound proteins as occurs in the VP16-inducedcomplex.

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FIG. 8. Models of HCF-1 binding to DNA in chromatin. (A) Hypothetical structure of HCF-1 bound to chromatin in cartoon form. In this model, HCF-1 is targeted to the DNA (black) in chromatin by its VP16 interaction or Kelch domain (dark green) through protein-protein interaction with a DNA-binding protein or protein complex (red). Other regions of HCF-1 $---$ the basic region (+), acidic region ( $-$ ), HCF-1_N-HCF-1_C association region (light green), and HCF-1_C-HCF-1_N association region (kidney shape with arrows) $---$ are shown in shades of green. Hypothetical effectors of HCF-1, proteins X and Y, are shown in shades of blue. (B and C) Alternative models for HCF-1 binding to chromatin. (B) HCF-1 associates with a single abundant species labeled $alpha$ (red) through its VP16 interaction domain. A multiplicity of other factors (yellow) may associate with and perhaps stabilize the association with the $alpha$ species in chromatin. (C) HCF-1 associates with different DNA-binding proteins (three, $alpha$ , $beta$ , and $gamma$ , are shown in the figure), any one member of which need not be abundant, but may bind DNA in different transcription factor (yellow) contexts.

This view of HCF-1 function suggests that, by targeting HCF-1 to specific DNA-bound regulatory proteins, the HCF-1 VP16 interactiondomain is responsible for providing regulatory specificity. Otherregions of HCF-1 are also essential, however, for its activity.For example, the HCF-1 basic region is necessary to promote cellproliferation (28). Because there is no evidence from our studiesthat these other regions of HCF-1 naturally bind to DNA eitherdirectly or indirectly, we suggest that they function by associatingwith other non-DNA-binding proteins (e.g., X and Y in Fig. 8A).An attractive model is that hypothetical basic region- and HCF-1_C-associatedproteins are enzymes that regulate, for example, chromatin structureor transcription factor function. With the HCF-1_C subunit, sucha candidate effector protein is the cell cycle-regulatory proteinphosphatase 1, which can bind to the carboxy-terminal HCF-1_C subunit(1). The basic region has not been shown to associate withany such enzymatic activities but instead is thought to associatewith the DNA-binding proteins GABP (26) and Sp1 (8). Becausethe basic region is not required for HCF-1 binding to chromatin,however, HCF-1 association with GABP or Sp1 is probably not essentialfor HCF-1 to bind to chromatin. Nevertheless, it may associatewith these two proteins once brought to the DNA through its VP16interaction domain or a minor population of HCF-1 not detectedin our study may associate with chromatin through theseproteins.

The findings that a single structural element of HCF-1 $---$ its VP16 interaction domain $---$ probably brings HCF-1 to the DNA by stoichiometricassociation with a DNA-binding protein(s) and that HCF-1 is veryabundant in the cell $---$ over 100,000 copies in a typical tissue culturecell $---$ have important implications for our understanding of thenature of the molecular target or targets of HCF-1. If the HCF-1VP16 interaction domain associates with a single species in thecell, as suggested by the hypothetical $alpha$ protein in Fig. 8B, thisspecies must be equally abundant. Proteins such as LZIP and ZF,which are present at very low levels in tissue culture cells (14,15), do not satisfy this criterion. We favor a second modelshown in Fig. 8C, in which HCF-1 associates with a large familyof DNA-binding proteins, of which any one member need not be abundant.Such a model would be consistent with functional association ofHCF-1 with proteins such as LZIP and ZF, which share the shortand degenerate (D/E)HXY HCF-1-binding motif. If true, this modelwould suggest that HCF-1 may function like coregulatory proteinssuch as the coactivators p300 and CREB-binding protein and thecorepressor mSin3, each of which associates with many differentDNA-binding transcriptional regulators (see references 2, 6,and 24).

Whichever model is correct, the finding that the wild-type HCF-1_N subunit lacking a canonical NLS (12) is both nuclear andchromatin bound suggests that, as with VP16, HCF-1 can associatewith its DNA-binding target protein(s) off of the DNA and $---$ perhapsin contrast to VP16 (see reference 12) $---$ bring HCF-1 to the nucleus.Consistent with this hypothesis, the HCF-1_N/P134S subunit, whichfails to associate with putative target proteins, is apparentlyneither chromatin bound nor nuclear (Fig. 3). The chromatin associationof wild-type HCF-1_N subunits explains why the HCF-1_N1011382-450protein, which lacks the NLS and does not associate with the HCF-1_Csubunit, can still rescue the temperature-induced tsBN67 cellproliferation defect (28).

Surprisingly, it is the very ability of HCF-1 to bind to chromatin that is temperature sensitive in the tsBN67 cell line,and loss of chromatin association precedes temperature-inducedarrest of tsBN67 cell proliferation. These results suggest thatthe temperature-sensitive cell proliferation defect of tsBN67cells results from the loss of HCF-1_P134S association with chromatinat the nonpermissive temperature. Both the loss of HCF-1_P134Schromatin association (Fig. 7) and the delayed loss of cell proliferation(7), however, require cell proliferation itself, suggestingthat they are each the result of an active growth process in themutant tsBN67cells.

The different time courses of HCF-1_P134S dissociation from chromatin (up to 18 h) and cell proliferation arrest (36 to 48h) upon transfer of tsBN67 cells to the nonpermissive temperaturebegin to reveal a cascade of events that leads to the arrest oftsBN67 cell proliferation. Perhaps HCF-1 dissociation from chromatinis delayed in asynchronous cells at the nonpermissive temperaturebecause it occurs during a particular phase of the tsBN67 cellcycle. Such a property would explain why proliferation is requiredfor dissociation of HCF-1 from chromatin and why there is a lagof about one cell cycle (i.e., about 12 to 18 h) for full lossof HCF-1 chromatin association (Fig. 6).

The results described here, together with the role of HCF-1 in HSV-1 VP16-induced transcriptional activation, suggest thatHCF-1 is a new player in transcriptional control of cell proliferation.HCF-1 may well have activities similar to those of better-understoodregulators of cell proliferation that, like HCF-1, are recruitedto the DNA by sequence-specific DNA-binding proteins. Two prominentexamples are the Rb protein, which associates with E2F and recruitshistone deacetylases (4, 19, 22), and mSin3, which associateswith numerous DNA-binding proteins and also recruits deacetylases(2, 24). Unlike these complexes, however, which repress cellproliferation, a putative HCF-1 complex promotes cell proliferationbecause loss of HCF-1 function leads to an arrest of cell proliferation.Thus, similar to its function as a viral transcriptional coactivator,HCF-1 may be a coactivator of transcription in uninfected cells.Consistent with this hypothesis, HCF-1 can enhance transcriptionalactivation by LZIP in transient-expression assays (17, 18).

Although the experiments described here have revealed similarities between HCF-1 and transcriptional regulatory proteins suchas Rb, the association of VP16 with HCF-1 and the DNA tumor virusearly proteins such as the adenovirus E1A protein and simian virus40 T-antigen proteins with Rb suggest opposing strategies of virus-hostcell interaction. The DNA tumor virus early proteins are synthesizedde novo upon infection, and by stoichiometric association theyinactivate Rb to promote infected-cell entry into S phase. Incontrast, VP16 is not synthesized de novo early in infection butinstead is brought in by the infecting virion(s), where thereare only 500 to 1,000 molecules of VP16 per virion (9) comparedto the estimated 100,000 molecules of HCF-1. Thus, unlike howE1A or T antigen inactivate the Rb protein early in infection,VP16 probably does not inactivate endogenous HCF-1 early in infectionand indeed may have little effect on its normal functions. Thus,rather than commandeer the cell, as do E1A and T antigen, VP16may associate with HCF-1 surreptitiously and use productive associationas one indication for whether the cellular environment is appropriateto promote lyticinfection.

	ACKNOWLEDGMENTS

We are indebted to J. Méndez for many helpful discussions concerning protein binding to chromatin and the small-scale chromatinisolation procedure; J. Lees for advice on the quantitation ofHCF-1; T. Nishimoto for BHK21 and tsBN67 cells; members of theHerr laboratory for helpful discussions; N. Hernandez, E. Julien,J. Méndez, and W. Tansey for critical readings of the manuscript;J. Duffy and P. Renna for photography; and J. Reader for helpin preparation of themanuscript.

This study was funded by U.S. Public Health Service grants GM54598 andCA13106.

	FOOTNOTES

^* Corresponding author. Mailing address: Cold Spring Harbor Laboratory, P.O. Box 100, 1 Bungtown Rd., Cold Spring Harbor, NY11724. Phone:(516) 367-8401. Fax: (516) 367-8454. E-mail: herr{at}cshl.org.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Kumar-Sinha, C., Varambally, S., Sreekumar, A., Chinnaiyan, A. M. (2002). Molecular Cross-talk between the TRAIL and Interferon Signaling Pathways. J. Biol. Chem. 277: 575-585 [Abstract] [Full Text]
Lee, S., Herr, W. (2001). Stabilization but Not the Transcriptional Activity of Herpes Simplex Virus VP16-Induced Complexes Is Evolutionarily Conserved among HCF Family Members. J. Virol. 75: 12402-12411 [Abstract] [Full Text]

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