Histone Deacetylase 4 Possesses Intrinsic Nuclear Import and Export Signals

doi:10.1128/MCB.21.17.5992-6005.2001

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Molecular and Cellular Biology, September 2001, p. 5992-6005, Vol. 21, No. 17
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.17.5992-6005.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Histone Deacetylase 4 Possesses Intrinsic Nuclear Import and Export Signals

Audrey H. Wang and Xiang-Jiao Yang^*

Molecular Oncology Group, Department of Medicine, McGill University Health Center, Montréal, Quebec H3A 1A1, Canada

Received 27 November 2000/Returned for modification 16 January 2001/Accepted 30 May 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Nucleocytoplasmic trafficking of histone deacetylase 4 (HDAC4) plays an important role in regulating its function, and bindingof 14-3-3 proteins is necessary for its cytoplasmic retention.Here, we report the identification of nuclear import and exportsequences of HDAC4. While its N-terminal 118 residues modulatethe nuclear localization, residues 244 to 279 constitute an authentic,strong nuclear localization signal. Mutational analysis of thissignal revealed that three arginine-lysine clusters are necessaryfor its nuclear import activity. As for nuclear export, leucine-richsequences located in the middle part of HDAC4 do not functionas nuclear export signals. By contrast, a hydrophobic motif (MXXLXVXV)located at the C-terminal end serves as a nuclear export signalthat is necessary for cytoplasmic retention of HDAC4. This motifis required for CRM1-mediated nuclear export of HDAC4. Furthermore,binding of 14-3-3 proteins promotes cytoplasmic localization ofHDAC4 by both inhibiting its nuclear import and stimulating itsnuclear export. Unlike wild-type HDAC4, a point mutant with abrogatedMEF2-binding ability remains cytoplasmic upon exogenous expressionof MEF2C, supporting the notion that direct MEF2 binding targetsHDAC4 to the nucleus. Therefore, HDAC4 possesses intrinsic nuclearimport and export signals for its dynamic nucleocytoplasmic shuttling,and association with 14-3-3 and MEF2 proteins affects such shuttlingand thus directs HDAC4 to the cytoplasm and the nucleus,respectively.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

How protein functions are regulated in vivo is a fundamental issue relevant to various biological processes. Lysine acetylationhas recently emerged as a major form of posttranslational modificationthat regulates functions of histones, nonhistone chromosomal proteins,and transcription factors (8, 21, 29, 52, 54). Acetylationof histones and other chromosomal proteins regulates chromatinactivities in transcription, replication, and recombination (3,38, 42, 55, 62). Histone deacetylases (HDACs) are theenzymes responsible for reversing the acetylation of histonesand other proteins. According to sequence homology and time ofidentification, mammalian HDACs can be divided into three classes.Class I HDACs (HDAC1, HDAC2, HDAC3, and HDAC8) show high similarityto the yeast deacetylase Rpd3 (4, 9, 12, 22, 56, 57,65, 66). Class II HDACs (HDAC4, HDAC5, HDAC6, and HDAC7) possesscatalytic domains significantly homologous to that of yeast Hda1(13, 19, 27, 43, 48, 59, 60). Class III is comprisedof proteins with catalytic domains similar to that of the yeastNAD⁺-dependent deacetylase Sir2 (15, 24, 31, 49).

Compared to class I deacetylases, much less is known about the second class (8). HDAC4, HDAC5, and HDAC7 are homologous,with their Hda1-related domains located in the C-terminal parts,whereas HDAC6 possesses tandem Hda1-related domains (13, 19,27, 43, 59, 60). Like class I members, class II HDACs(except HDAC6) have been found to be corepressors recruited fortranscriptional repression. The MEF2 transcription factors interactwith HDAC4, HDAC5, HDAC7, and their related protein monocyte enhancerfactor 2 (MEF2)-interacting transcription repressor (MITR) (alsoknown as HDAC-related protein) to repress transcription (11,32, 35, 43, 50, 60, 69). Moreover, this interactionis signal dependent and regulated during muscle differentiation(11, 35, 36, 67). HDAC4, HDAC5, and HDAC7 also interactwith the nuclear receptor corepressors SMRT and N-CoR to represstranscription (23, 27).

How are functions of different deacetylases regulated in vivo? Emerging evidence suggests that cellular compartmentalizationis one major regulatory mechanism for class II HDACs (8, 28).Active nucleocytoplasmic shuttling has been shown for HDAC4 (20,43, 61), HDAC5 (40, 41), HDAC6 (58), and HDAC7 (11).Moreover, such shuttling is tightly controlled. 14-3-3 proteinsdirectly bind to HDAC4 and HDAC5 and negatively regulate theirroles in transcriptional repression (20, 40, 61). 14-3-3binding to HDAC5 and perhaps to its homologs (i.e., HDAC4 andHDAC7) plays an important role in regulating functions of MEF2during muscle differentiation (11, 36, 40, 41, 53).Three serine residues of HDAC4 (i.e., S246, S467, and S632) mediateits binding to 14-3-3 proteins (20, 61). Unlike wild-typeHDAC4, the triple mutant S246/467/632A is completely defectivein 14-3-3 binding and is localized to the nucleus (20, 61),indicating that 14-3-3 binding is necessary for retaining HDAC4in the cytoplasm. However, it remains unclear whether 14-3-3 bindingalone is sufficient for cytoplasmic retention ofHDAC4.

While characterizing the interesting link between HDAC4 and 14-3-3 proteins, we unexpectedly found that the mutant 118-1084/S246/467/632A,the triple mutant which lacks the N-terminal 118 residues of HDAC4,was mainly cytoplasmic or pancellular. To understand this intriguingfinding, we engineered and analyzed various HDAC4 mutants, whichhas led to the identification of sequence elements that are importantfor nucleocytoplasmic trafficking of HDAC4. While the N-terminal118 residues and MEF2-binding site of HDAC4 modulate its nuclearlocalization, residues 244 to 279 constitute an authentic, tripartitenuclear localization signal (NLS) and a C-terminal hydrophobicmotif serves as a functional nuclear export signal (NES). ThisNES is required for CRM1-mediated nuclear export of HDAC4. Furthermore,both 14-3-3 binding and the NES-mediated nuclear export are requiredfor cytoplasmic retention of HDAC4. We propose that subcellulardistribution of HDAC4 is controlled by multiple mechanisms invivo. Such a regulatory scheme may provide flexibility for fine-tuningbiological functions ofHDAC4.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Molecular cloning. Expression plasmids for HDAC4 and some deletion mutants have been described previously (60, 61). Additional HDAC4 mutantswere generated by PCR with Expand (Roche) thermostable DNA polymeraseor by site-directed mutagenesis with single-stranded uracil-containingtemplates and T7 DNA polymerase. DNA sequencing was performedwith T7 Sequenase 2.0 (Amersham Pharmacia Biotech) for confirmationof mutations. Green fluorescent protein (GFP) constructs werederived from pEGFP-C2(Clontech).

Green fluorescence microscopy. NIH 3T3 and 293 cells were transfected with plasmids expressing GFP fusion proteins using SuperFect transfection reagent (Qiagen)(5, 60). At 16 h after transfection, living cells were analyzedby GFP fluorescence microscopy as described (61). Fluorescenceimages were collected using a charge-coupled device camera (Q-imaging,Inc.) linked to a computer running Northern Eclipse (version 5.0;Empix Imaging) and exported for further processing with AdobePhotoshop. Alternatively, cells were fixed with formaldehyde andcounterstained with Hoechst 33528 to visualize the nuclei (61);Hoechst and green fluorescence images were subsequentlycollected.

Immunofluorescence microscopy. To assess effects of MEF2 binding on subcellular localization of HDAC4 and its mutants, MEF2C expression plasmid was transfectedinto NIH 3T3 cells along with mammalian expression plasmids forHDAC4 or its mutants fused to GFP. To detect the expression ofMEF2C, cells were fixed with formaldehyde 16 h after transfection,incubated with anti-MEF2C antibody, and stained with Cy3 anti-rabbitimmunoglobulin G antibody (Jackson Immunoresearch) as previouslydescribed (37, 61). Cells were counterstained with Hoechst33528 to visualize the nuclei. Expression of GFP fusion proteinswas determined by green fluorescence microscopy. Similarly, effectsof exogenous CRM1 on subcellular localization of HDAC4 mutantsweredetermined.

Protein-protein interaction. To analyze interaction of the MEF2C mutant M178 with HDAC4 mutants, in vitro maltose-binding protein (MBP) binding assayswere carried out as described (60). For analysis of intra- orintermolecular interaction among HDAC4 molecules, its fragmentswere expressed as MBP fusion proteins in Escherichia coli, immobilizedon amylose agarose (New England Biolabs), and incubated with HDAC4or its fragments synthesized in vitro by use of a TNT-T7 coupledreticulocyte lysate system (Promega) in the presence of L-[³⁵S]methionine (Amersham Pharmacia Biotech). Agarose beads werewashed three times with buffer B (20 mM Tris-HCl [pH 8.0], 10%glycerol, 5 mM MgCl₂, 0.1% NP-40, protease inhibitors) containing0.15 M KCl and once with buffer B containing 0.5 M KCl. Boundproteins were then analyzed by reducing sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and autoradiography as previouslydescribed (60).

Western blotting analysis. Expression of GFP fusion proteins was also confirmed by Western blotting analysis of total cell extracts as previously described(6, 60). 293 cells were transfected with plasmids expressingGFP fusion proteins using SuperFect transfection reagent (Qiagen)(5, 60). At 16 h after transfection, cells were washed twicewith ice-cold phosphate-buffered saline (PBS) and collected inice-cold buffer B containing 0.15 M KCl or in buffer H (20 mMHEPES [pH 7.6], 20% glycerol, 150 mM NaCl, 1.5 mM MgCl₂, 0.2 mMEDTA, 0.1% Triton X-100, 25 mM NaF, 10 mM $beta$ -glycerophosphate,1 mM dithiothreitol, protease inhibitors). After being rotatedat 4°C for 20 min, the cell lysates were cleared by high-speedcentrifugation at 4°C, and the supernatants were collected astotal cell extracts. For immunoblotting, the total cell extracts(~10 µg/lane) were resolved by reducing SDS-PAGE, electro-transferredto nitrocellulose membrane, and subsequently immunoblotted withanti-GFP antibody (Santa Cruz Biotechnology; sc-8334). For blockingand antibody incubation, PBS containing 20% horse serum (GG free;Gibco BRL) and 0.15% Tween 20 (Sigma) was used. For washing, PBSwith 0.15% Tween 20 was used. Blots were developed with Supersignalchemiluminescent substrate(Pierce).

BLAST search. Amino acid sequence homology searches were performed at the NCBI BLAST server (http://www.ncbi.nlm.nih.gov/BLAST/) using PSI-BLASTwith the matrix BLOSUM62 (1).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Compared to the yeast deacetylase Hda1, HDAC4 can be divided into three parts: an extended N-terminal region (residues 1 to620), an Hda1-related deacetylase domain (residues 621 to 1039),and a small C-terminal module (residues 1040 to 1084) (Fig. 1A).The extended N-terminal region has been found to interact withMEF2 and 14-3-3 proteins (20, 43, 60, 61), whereas thefunction of the small C-terminal module remains elusive.

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FIG. 1. Role of the N-terminal 118 residues of HDAC4 in regulating its nuclear localization. (A) Schematic illustration of HDAC4 and mutants. For HDAC4, 14-3-3 binding sites (S246, S467, and S632) and the Hda1-homology domain are depicted by boxes. In the triple mutants TM1 to TM4, the three serine residues critical for 14-3-3 binding are changed to alanine. Subcellular localization of HDAC4 and mutants is summarized at right: C, predominantly cytoplasmic; N, predominantly nuclear; P, pancellular. Shown at the lower part of the panel is the sequence comparison between homologous regions of HDAC4 (residues 90 to 142) and MAG1 (residues 504 to 556), with identical or conserved residues shaded. (B and C) Representative green fluorescence images of living (B) or fixed (C) NIH 3T3 cells expressing GFP or its fusion proteins. Cells were transfected with expression plasmids for GFP or its fusion proteins and subsequently analyzed by fluorescence microscopy 16 h after transfection. (B) Living cells were directly used for microscopic analysis. (C) Transfected cells were fixed with formaldehyde, counterstained with Hoechst 33528 and analyzed by green fluorescence microscopy (top), with corresponding Hoechst fluorescence images also taken (bottom). (D) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for indicated GFP fusion proteins, and total cell extracts were analyzed by immunoblotting with anti-GFP antibody.

Role of the N-terminal 118 residues of HDAC4 in modulating its nuclear localization. We and others have previously shown that the HDAC4 triple mutant TM1 (Fig. 1A) is completely defective in 14-3-3 binding andthus predominantly nuclear (20, 61). As reported, GFP-HDAC4and -TM1 were cytoplasmic and nuclear, respectively, whereas GFPitself was pancellular in NIH 3T3 cells (Fig. 1B and C). Alsoconsistent with published reports (43, 61), the mutant 118-1084was predominantly cytoplasmic (Fig. 1 and data not shown). Unexpectedly,we found that unlike GFP-TM1, GFP-TM2 was either cytoplasmic orpancellular (Fig. 1), suggesting that the N-terminal 118 residuesare involved in regulating nuclear localization of HDAC4. BLASTsearches revealed that residues 90 to 142 of HDAC4 show limitedsequence similarity to the GTP-binding protein MAG1 (Fig. 1A)(7, 63). To address whether the MAG1-related region of HDAC4is responsible for the observed difference between GFP-TM1 and-TM2, we engineered the mutants TM3 and TM4 fused to GFP (Fig.1A). As shown in Fig. 1B and C, unlike GFP-TM3, GFP-TM4 was moresimilar to GFP-TM1, suggesting that the MAG1-homology region maybe important for controlling nuclear localization of HDAC4. Aspreviously reported (61), GFP-TM1 was nuclear in most cells.By contrast, GFP-TM4 was found to be nuclear in 40 to 50% of thecells expressing this fusion protein (data not shown), suggestingthat the N-terminal 85 residues are also important for nuclearlocalization of HDAC4. To determine whether GFP fusion proteinsare expressed as expected, we performed Western blotting analysis.As shown in Fig. 1D, GFP fusion proteins with expected sizes weredetected. Taken together, these results indicate that the N-terminal118 residues of HDAC4 play an important role in modulating itsnuclearlocalization.

How do the N-terminal 118 residues of HDAC4 modulate its nuclear localization? To promote its nuclear localization, the N-terminal 118 residues of HDAC4 may: (i) be involved in inter- or intramolecularinteraction with HDAC4 itself (such interaction may affect theexposure of potential nuclear import or export sequences), (ii)interact with other nuclear proteins, or (iii) be (part of) anNLS. To distinguish among these possibilities, we first investigatedwhether the N-terminal part of HDAC4 mediates inter- or intramolecularinteraction with HDAC4 itself. For this, we analyzed differentHDAC4 deletion mutants (Fig. 2A) by in vitro binding assays usingMBP or its fusion proteins immobilized on amylose agarose. Asshown in Fig. 2B, no interaction was detectable between mutant315-1084 and MBP-1-326 (lanes 1 to 3). By contrast, mutant 1-326interacted with MBP-1-326 but not MBP itself (lanes 4 to 6). Totest whether the N-terminal 118 residues are essential for thisinteraction, we tested the deletion mutants 1-208 and 1-114. Asshown in Fig. 2C, neither mutant was retained by MBP-1-326, suggestingthat residues 118 to 326 may be responsible for the interaction.In agreement with this, MBP-1-326 interacted with HDAC4, mutant118-1084 and mutant 118-326 (Fig. 2D), suggesting that residues118 to 326 of HDAC4 constitute a dimerization domain. Taken together,these results indicate that the N-terminal 118 residues of HDAC4do not appear to be involved in inter- or intramolecular interactionwith HDAC4 itself.

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FIG. 2. Mapping the dimerization domain of HDAC4. (A) Schematic representation of HDAC4 and deletion mutants. Motifs or domains are depicted by boxes as in Fig. 1A. (B to D) Interaction among HDAC4 proteins. HDAC4 deletion mutants were expressed as MBP fusion proteins in E. coli, immobilized on amylose agarose and incubated with HDAC4 or deletion mutants synthesized in vitro in the presence of L-[³⁵S]methionine. Agarose beads were washed three times with buffer B-0.15 M KCl and once with buffer B-0.5 M KCl. Bound proteins were separated by SDS-PAGE and subsequently detected by autoradiography. Input represents 20% of the ³⁵S-labeled protein used for each binding assay. Migrating positions of molecular markers are shown at the left of each panel.

As discussed above, the N-terminal 118 residues may interact with other nuclear proteins and thereby stimulate nuclear localizationof HDAC4. Two proteins are known to have the potential to interactwith the N-terminal part of HDAC4. Although the exact bindingsite has not been mapped, HDAC1 has been shown to be associatedwith MITR, a corepressor with sequence similarity to the N-terminalpart of HDAC4 (50). Adenovirus E1A C-terminal-binding protein(CtBP) has also been shown to interact with HDAC4, and its N-terminal118 residues possesses a putative CtBP-binding site (68). Totest whether HDAC1 or CtBP modulates subcellular localizationof HDAC4, we examined effects of their overexpression on intracellulardistribution of GFP-HDAC4 by fluorescence microscopy. The resultsindicated that overexpression of HDAC1 or CtBP had minimal effectson the cytoplasmic localization of GFP-HDAC4 (data not shown),suggesting that neither HDAC1 nor CtBP is involved in modulatingintracellular localization of HDAC4. It still remains possible,however, that an unidentified protein may interact with the N-terminal118 residues of HDAC4 and thereby modulate its intracellulardistribution.

To investigate whether the N-terminal 118 residues of HDAC4 constitute (or are part of) an NLS, we examined subcellular distributionof the HDAC4 deletion mutants 1-118 and 1-165 expressed as GFPfusion proteins (Fig. 3A). As shown in Fig. 3B, both mutants werepartially enriched in the nucleus, suggesting that the N-terminal118 residues of HDAC4 only possess weak nuclear targeting ability.This region does not show any sequence resemblance to classicalarginine-lysine-rich nuclear import signals, raising the possibilitythat a yet-unknown protein interacts with this region of HDAC4and regulates its subcellular localization (see Discussion).

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FIG. 3. Mapping the NLS of HDAC4. (A) Schematic representation of HDAC4 and deletion mutants. Motifs or domains are depicted by boxes as in Fig. 1A. Also indicated are two arginine-lysine-rich regions: RK1 (residues 132 to 184) and RK2 (residues 242 to 283). (B) Representative green fluorescence images of living cells expressing HDAC4 mutants fused to GFP. NIH 3T3 cells were transfected with expression plasmids for indicated GFP fusion proteins and analyzed by live green fluorescence microscopy. (C) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for indicated GFP fusion proteins, and total cell extracts were analyzed by immunoblotting with anti-GFP antibody.

Identification of an authentic HDAC4 NLS. The distinct localization between GFP-TM1 (nuclear [Fig. 1]) and GFP-1-165 (partially enriched in the nucleus [Fig. 3]) furthersuggests that there is a strong NLS within residues 166 to 1084.Consistent with this, HDAC4 possesses two arginine-lysine-richsequences (RK1 and RK2) (Fig. 3A). To further understand how nucleocytoplasmicdistribution of HDAC4 is controlled, we decided to map its NLS.To take a systematic approach, we first analyzed the deletionmutants 1-208, 1-266, 1-326, and 1-669 expressed as GFP fusionproteins (Fig. 3A). As shown in Fig. 3B, the localization of mutant1-208 was similar to that of mutants 1-114 and 1-165, suggestingthat RK1 is not an NLS. Distinct from mutant 1-208, mutant 1-266was pancellular (Fig. 3B). One explanation for this is that 14-3-3binding to S246 of mutant 1-266 counteracts the weak nuclear targetingactivity that the N-terminal 118 residues exhibit. Unlike mutant1-266, the mutants 1-326 and 1-669 were exclusively or predominantlynuclear, indicating that residues 267 to 326 are important forthe nuclear localization activity. Consistent with this, the mutant206-326 was exclusively nuclear. Together, these results suggestthat RK2 may possess an authentic NLS. To further map this NLS,we constructed and analyzed the mutants 206-279, 206-266, 244-326,and 263-326 (Fig. 3A). These mutants were designed according tothe sequence of RK2 (residues 242 to 283, Fig. 4A). While mutants206-279 and 244-326 were nuclear, mutants 206-266 and 263-326were mainly pancellular (Fig. 3B), indicating that residues 244to 279 are important for the nuclear localization activity. Totest whether this region is sufficient, we examined the mutant244-279 expressed as a GFP fusion protein (Fig. 3A). As shownin Fig. 3B, this mutant was exclusively nuclear, indicating thatresidues 244 to 279 of HDAC4 are capable of directing GFP to thenucleus. Western blotting analysis with anti-GFP antibody revealedthat the deletion mutants used for mapping the NLS were correctlyexpressed (Fig. 3C). Taken together, these mapping data indicatethat residues 244 to 279 of HDAC4 constitute an authentic NLS.

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FIG. 4. Mutational analysis of the NLS. (A) Illustration of mutant 206-326 and its point mutants. The amino acid sequence of residues 242 to 283 of HDAC4 is listed, with potentially important arginine-lysine residues shown in boldface type. Residues important for 14-3-3 binding are labeled with asterisks. The point mutants PM1 to PM4 were derived from the deletion mutant 206-326 by substitution of indicated arginine-lysine residues. (B) Representative green fluorescence images of living NIH 3T3 cells expressing PM1 to PM4 fused to GFP. Cells were transfected with expression plasmids for indicated GFP fusion proteins, and green fluorescence microscopy was performed with living cells. For each mutant, two images are shown to illustrate distinct localization in different cells. (C) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for indicated GFP fusion proteins, and cell extracts were analyzed by immunoblotting with anti-GFP antibody.

Point mutational analysis of the HDAC4 NLS. To further define the NLS, we sought to identify its critical residues. Residues 244 to 279 possess three clusters of arginine-lysineresidues (Fig. 4A). To test whether these clusters are requiredfor the nuclear targeting activity, we derived the point mutantsPM1 to PM4 from the deletion mutant 206-326 by mutating arginine-lysineresidues. GFP fusion proteins were expressed and analyzed by greenfluorescence microscopy. As shown in Fig. 4B, unlike mutant 206-326,PM1 to PM4 were pancellular, cytoplasmic, or partially enrichedin the nucleus. Western blotting analysis revealed that thesepoint mutants were correctly expressed (Fig. 4C). Therefore, thethree clusters of arginine-lysine residues are all necessary forthe nuclear localization of mutant 206-326. This also impliesthat the NLS of HDAC4 istripartite.

Nuclear export activity of leucine-rich sequences of HDAC4. We wondered why GFP-TM2 (Fig. 1) was not localized to the nucleus, although it possesses the strong NLS just identified. Cytoplasmiclocalization of HDAC4 is sensitive to treatment with leptomycinB (LMB) (43, 61). LMB is a specific inhibitor of the nuclearexport receptor CRM1 (14, 30, 46, 51), so HDAC4 is subjectto active nuclear export. 14-3-3 binding to HDAC4 promotes itscytoplasmic retention (20, 43, 61). 14-3-3 proteins aredimeric, and each monomer is known to possess an active NES (34,47). Therefore, one explanation for the active nuclear exportof HDAC4 is that it binds to 14-3-3 proteins and is subsequentlytargeted to the cytoplasm through LMB-sensitive nuclear export.Alternatively, HDAC4 may possess an intrinsic NES that directsit to the cytoplasm. Since its 14-3-3 binding sites are impaired,the cytoplasmic localization of GFP-TM2 (Fig. 1) supports thelatter possibility. However, this does not exclude the former.With this reasoning in mind, we dissected the underlying mechanismsby which HDAC4 is exported from thenucleus.

Some leucine-rich sequences are known export signals recognized by the nuclear export receptor CRM1 (45). HDAC4 possessesseveral leucine-rich sequences (Fig. 5A). In particular, residues429 to 438 match exactly the NES consensus sequence derived fromvarious known export signals (2). In light of this observation,we expressed and analyzed the HDAC4 mutant 315-488 as a GFP fusionprotein. As shown in Fig. 5B, this mutant was partially enrichedin the cytoplasm. Since this mutant contains a 14-3-3 bindingsite, we decided to investigate whether its partial enrichmentin the cytoplasm is due to 14-3-3 binding. For this, S467 wassubstituted with alanine to generate the mutant 315-488/S467A.This mutant was found to be pancellular (Fig. 5B). Without activenuclear import and export, such a localization is expected sincethis mutant may be able to passively diffuse through nuclear pores(18). Western blotting analysis with anti-GFP antibody indicatedthat both 315-488 and 315-488/S467A were well expressed (Fig.5C). Together, these results suggest that the enrichment of mutant315-488 in the cytoplasm is due to 14-3-3 binding, implying thatthe leucine-rich sequences of HDAC4 do not have nuclear exportactivity.

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FIG. 5. Nuclear export activity of leucine-rich sequences of HDAC4. (A) Amino acid sequence of leucine-rich motifs of HDAC4, with leucine and methionine residues shown in boldface type. The consensus sequence of known leucine-rich export signals is also shown, with X denoting any amino acid residue. (B) Representative green fluorescence images of living cells expressing mutant 315-488 and its point mutant fused to GFP. NIH 3T3 cells were transfected with expression plasmids for the mutants, and green fluorescence microscopy was performed with living cells. (C) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for GFP-315-488 and -315-488/S467A, and total cell extracts were analyzed by immunoblotting with anti-GFP antibody.

Mapping an NES to the C-terminal end of HDAC4. To investigate whether other sequences of HDAC4 may exhibit nuclear export activity, we examined subcellular localizationof the deletion mutants 206-1084, 315-1084, and 621-1084 fusedto GFP (Fig. 6A). As shown in Fig. 6B, these mutants were predominantlycytoplasmic. Western blotting analysis with anti-GFP antibodyindicated that these deletion mutants were expressed as expected(Fig. 6C, lanes 1 to 3). To test whether the S632 14-3-3 bindingsite contributes to the cytoplasmic localization of mutant 621-1084,we analyzed the mutants 531-1084 and 531-1084/S632A expressedas GFP fusion proteins. Both mutants were found to be cytoplasmic(data not shown), suggesting that 14-3-3 binding is not the majormechanism by which mutant 621-1084 is sequestered to the cytoplasm.The cytoplasmic localization of mutant 621-1084 could be eitherthat it is not imported to the nucleus or that it is subject toactive nuclear export. To distinguish between these two possibilities,we utilized the nuclear export inhibitor LMB since HDAC4 is knownto be exported in an LMB-sensitive manner (43, 61). As shownin Fig. 6D, LMB treatment inhibited the predominantly cytoplasmiclocalization of mutant 621-1084, indicating that mutant 621-1084is subject to active nuclear export. The pancellular localizationafter LMB treatment is perhaps due to passive diffusion throughnuclear pores (18). Therefore, residues 621 to 1084 possessan intrinsic NES.

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FIG. 6. Mapping intrinsic NES of HDAC4. (A) Schematic illustration of HDAC4 and its deletion mutants. Motifs or domains are depicted by boxes as in Fig. 1A. Subcellular localization of HDAC4 and mutants is summarized at right. (B and E) Representative green fluorescence images of living cells expressing HDAC4 and its deletion mutants fused to GFP. NIH 3T3 cells were transfected with expression plasmids for indicated GFP fusion proteins, and green fluorescence microscopy was performed with living cells. (C and F) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for indicated GFP fusion proteins, and total cell extracts were analyzed by immunoblotting with anti-GFP antibody. (D and G) Effect of LMB on subcellular distribution of indicated GFP fusion proteins expressed in NIH 3T3 cells. After initial examination for green fluorescence, living cells expressing the indicated fusion proteins were treated with LMB (10 ng/ml), and their green fluorescence images were taken at indicated times. Under similar conditions, LMB had minimal effects on subcellular localization of GFP itself (data not shown).

To map the NES, we first considered whether it is located at the small C-terminal domain (residues 1040 to 1084) since thisregion is missing in Hda1 (Fig. 6A). This small domain was thusdeleted to generate the mutant 1-1040 fused to GFP (Fig. 6A).This fusion protein was predominantly nuclear (Fig. 6E), indicatingthat the small C-terminal domain is indeed required for cytoplasmiclocalization of HDAC4. Since this mutant possesses intact 14-3-3binding sites (20, 61), this exciting finding also indicatesthat 14-3-3 binding is not sufficient for retaining HDAC4 in thecytoplasm. To further define the small C-terminal domain, smalldeletions from the C-terminal end were engineered to express themutants 1-1069, 1-1061, and 1-1055 as GFP fusion proteins (Fig.6A). The mutant 1-1069 was predominantly cytoplasmic (Fig. 6E),suggesting that residues 1070 to 1084 of HDAC4 are dispensablefor its cytoplasmic localization. The two mutants 1-1061 and 1-1055were predominantly nuclear (Fig. 6E), indicating that residues1062 to 1069 are essential for cytoplasmic retention of HDAC4.These results also imply that residues 1040 to 1069 of HDAC4 mayconstitute an NES. To test this hypothesis, we expressed the mutant1044-1069 as a GFP fusion protein (Fig. 6A). As shown in Fig.6E, this fusion protein was predominantly cytoplasmic. On theother hand, mutant 621-1040 was pancellular (Fig. 6E). Westernblotting analysis with anti-GFP antibody indicated that thesedeletion mutants were correctly expressed (Fig. 6C, F). Together,these results indicate that residues 1044 to 1069 of HDAC4 functionas anNES.

We also examined the mutants 315-1040 and 206-1040 expressed as GFP fusion proteins (Fig. 6A). Different from mutant 315-1084(Fig. 3B), mutant 315-1040 was pancellular or cytoplasmic (Fig.6D). Unlike mutant 206-1084 (Fig. 3B), mutant 206-1040 was predominantlynuclear (Fig. 6D). The distinct localization between the mutants315-1040 and 206-1040 supports the aforementioned conclusion thatresidues 244 to 279 constitute an NLS (Fig. 3). The pancellularor cytoplasmic localization of mutant 315-1040 is expected sincethis mutant may be able to passively diffuse into the nucleusthrough nuclear pores and 14-3-3 binding to S467 and S632 of 315-1040may promote its active nuclear export. Western blotting analysiswith anti-GFP antibody indicated that mutants 206-1040 and 315-1040were correctly expressed (Fig. 6C, lanes 4 to 5). Together, theseresults underscore the importance of residues 1044 to 1069 forcytoplasmic retention ofHDAC4.

To determine whether residues 1044 to 1069 retain HDAC4 in the cytoplasm by nuclear export, we treated NIH 3T3 cells expressingGFP-1044-1069 with LMB. This fusion protein is small (~28 kDa)and does not appear to contain an NLS, so it can passively diffusethrough nuclear pores (18, 26). Therefore, this fusion proteinwould be expected to be pancellular if its nuclear export is inhibitedby LMB. As shown in Fig. 6G, upon LMB treatment, mutant 1044-1069became pancellular within 15 min, indicating that nuclear exportof mutant 1044-1069 is sensitive to LMB. Therefore, residues 1044to 1069 constitute an NES whose activity is LMB sensitive. SinceLMB is a CRM1-specific inhibitor (14, 30, 46, 51), CRM1may recognize thisNES.

Point mutational analysis of the HDAC4 NES. To further define the NES, we sought to identify its critical residues. Sequence inspection revealed that residues 1056 to1069 constitute a highly hydrophobic motif (Fig. 7A). Since CRM1is known to recognize leucine-rich or other hydrophobic motifs(45), residues 1056 to 1069 may constitute a functional NES.To determine which residues are important, we performed alaninescanning mutagenesis to generate mutants in which each nonalanineresidue was replaced with alanine (Fig. 7A). Fluorescence microscopicanalysis of these GFP fusion proteins revealed that substitutionof M1059, L1062, V1064, or V1066 of HDAC4 led to nuclear accumulationof the resulting mutants (Fig. 7B). Western blotting analysiswith anti-GFP antibody indicated that all point mutants were correctlyexpressed (Fig. 7C). Together, these results suggest that M1059,L1062, V1064, and V1066 are important for nuclear export of HDAC4.These residues constitute a hydrophobic motif, MXXLXVXV, whereX represents any amino acid residue.

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FIG. 7. Mutational analysis of the NES. (A) Amino acid sequences of residues 1056 to 1069 of HDAC4 and mutants. M1059, L1062, V1064, and V1066 of HDAC4 are labeled with asterisks. For the point mutants, substituted and unchanged residues are indicated by the letter A (for alanine) and hyphens, respectively. (B) Representative green fluorescence images of living cells expressing HDAC4 mutants fused to GFP. NIH 3T3 cells were transfected with expression plasmids for indicated GFP fusion proteins, and green fluorescence microscopy was performed with living cells. (C) Expression of GFP fusion proteins. 293 cells were transfected with expression plasmids for indicated GFP fusion proteins, and total cell extracts were analyzed by immunoblotting with anti-GFP antibody. The asterisk at right marks the expected migrating position.

CRM1 directs NES-mediated nuclear export of HDAC4. While the NES of HDAC4 is distinct from most known nuclear export sequences recognized by CRM1, its function appeared to beLMB sensitive (Fig. 6). This suggests that the NES may be regulatedby CRM1. To substantiate this, we sought to examine directly whetherCRM1 can mediate nuclear export of HDAC4 and how the NES is involved.It has been demonstrated that overexpression of CRM1 leads tonuclear exclusion of two transcription factors (17, 71). Sincewild-type HDAC4 is mainly cytoplasmic, we tested whether overexpressionof CRM1 can lead to nuclear exclusion of TM1 and S246/467A. WhileTM1 possesses no functional 14-3-3 binding sites, the double mutantS246/467A contains only one functional 14-3-3 binding site (S632[Fig. 1A]). Both mutants have been found to be predominantly nuclear(61). As shown in Fig. 8, exogenous expression of CRM1 promotedcytoplasmic localization of both mutants, suggesting that CRM1directs HDAC4 to the cytoplasm. To assess whether the NES of HDAC4is involved, we examined the mutants 1-1040 and L1062A. 14-3-3binding sites are intact in both mutants, but the NES is deletedin mutant 1-1040 (Fig. 6) and impaired by point mutation in L1062A(Fig. 7). As shown in Fig. 8, CRM1 overexpression had minimaleffects on the nuclear localization of these two mutants, indicatingthat the NES of HDAC4 is required for its CRM1-mediated nuclearexport.

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FIG. 8. Effects of overexpressed CRM1 on subcellular localization of HDAC4 mutants. An HA-CRM1 expression plasmid was transfected into NIH 3T3 cells along with mammalian expression plasmids for HDAC4 mutants fused to GFP. At 16 h after transfection, cells were fixed and stained with antihemagglutinin antibody to detect exogenous CRM1 (middle, red) by indirect immunofluorescence microscopy. Green fluorescence was used to determine subcellular localization of GFP fusion proteins (left) (green). The cells were counterstained with Hoechst 33528 to visualize nuclei (right) (blue). While endogenous CRM1 is enriched around the nuclear envelope, overexpressed CRM1 has been found to be pancellular or nuclear (17, 71).

Direct MEF2 binding targets HDAC4 to the nucleus. Identification of intrinsic nuclear import and export signals of HDAC4 further supports the notion that it is subject to dynamicnucleocytoplasmic shuttling. Binding of 14-3-3 proteins promotescytoplasmic localization of HDAC4 by affecting such dynamic shuttling(20, 40, 61). This led us to ask whether association ofother proteins also alters this shuttling. It has been shown thatthe HDAC4 mutant 118-1084 translocates to the nucleus upon exogenousexpression of MEF2A in HeLa cells (43). It was not proven, however,whether direct MEF2 binding is required for this nuclear targeting.To further understand how MEF2 may affect intracellular localizationof HDAC4, we first tested whether full-length HDAC4 is targetedto the nucleus upon exogenous expression of MEF2C in NIH 3T3 cells.As shown in Fig. 9, coexpression of MEF2C led to nuclear accumulationof GFP-HDAC4. We then asked whether the nuclear targeting of HDAC4requires its NLS and/or MEF2-binding site. To address this, weassessed whether coexpression of MEF2C affects subcellular localizationof the HDAC4 mutants 1-208 and 206-1084. While mutant 1-208 possessesthe MEF2-binding site (32, 35, 43, 50, 60), mutant 206-1084contains the NLS described above. In the absence of exogenousMEF2C, mutant 1-208 was partially enriched in the nucleus (Fig.3), whereas mutant 206-1084 was predominantly cytoplasmic (Fig.6). As shown in Fig. 9, expression of MEF2C promoted nuclear accumulationof mutant 1-208 but not mutant 206-1084, suggesting that MEF2directs HDAC4 to the nucleus in a manner dependent on its MEF2-bindingsite but not NLS.

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FIG. 9. Effects of exogenous MEF2C on nuclear localization of HDAC4 and mutants. The MEF2C expression plasmid was transfected into NIH 3T3 cells along with mammalian expression plasmids for GFP fusion proteins of HDAC4 or its mutants. At 16 h after transfection, cells were fixed and stained with anti-MEF2C antibody to detect MEF2C by indirect immunofluorescence microscopy (middle) (red). Green fluorescence was used to determine subcellular distribution of GFP fusion proteins (left) (green). The cells were counterstained with Hoechst 33528 to visualize nuclei (right) (white).

To further investigate whether direct MEF2 binding is essential for the nuclear targeting, we sought to analyze an HDAC4 pointmutant that is completely defective in MEF2 binding. For this,we first conducted mutational analysis of the MEF2-binding siteof HDAC4 to test whether point mutations can abrogate the MEF2binding and to identify residues critical for such binding. Weand others have located the MEF2-binding site to a small motifconserved among HDAC4, HDAC5, HDAC7, and MITR (Fig. 10A) (32,35, 43, 50, 60). Mutagenesis was thus performed to substitutepotentially important residues of this motif with alanine, andin vitro binding assays were utilized to assess how well eachmutant binds to MEF2. For binding assays, M178, an MEF2C mutantcontaining its N-terminal 178 residues (60), was expressed asan MBP fusion protein. As reported, HDAC4 interacted with MBP-M178but not MBP itself (Fig. 10B, lanes 1 to 3). Like wild-type HDAC4,the double mutant S168A/T169A interacted with M178 (lanes 4 to6), indicating that S168 and T169 of HDAC4 are not critical forMEF2 binding. By contrast, the double mutant V171A/K172A was unableto interact with M178 (lanes 7 to 9), suggesting that V171 and/orK172 is important for MEF2 binding. Consistent with this, V171Aweakly interacted with M178 (Fig. 10C, lanes 1 to 3), whereas K172Awas completely defective in binding to M178 (lanes 7 to 9). NeitherL175A (Fig. 10C, lanes 7 to 9) nor L175G (Fig. 10D, lanes 1 to 3)interacted with M178, indicating that L175 of HDAC4 is criticalfor MEF2 binding. In a similar fashion, V179, L180, and K182 ofHDAC4 were found to be involved in interaction with MEF2 (Fig.10D and E). Among the HDAC4 mutants analyzed, L175G is one whoseMEF2-binding ability is completely abolished.

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FIG. 10. Mutational analysis of the MEF2-binding site of HDAC4. (A) Sequence comparison of residues 166 to 184 of HDAC4 with the corresponding regions of HDAC5 and HDAC7. Identical or conserved residues are shaded, and L175 of HDAC4 is indicated by an asterisk. (B to E) Interaction of the MEF2C mutant M178 with HDAC4 and point mutants. MBP or MBP-M178 was immobilized on amylose agarose and tested for interaction with HDAC4 or mutants synthesized in vitro in the presence of [³⁵S]methionine. Bound proteins were separated by SDS-PAGE and subsequent autoradiography. Input represents 20% of the ³⁵S-labeled protein used for each binding assay. Migrating positions of molecular markers are shown at the left of each panel, whereas the positions of HDAC4 and its mutants are indicated by asterisks at right.

We next analyzed GFP-L175G by fluorescence microscopy. Like GFP-HDAC4, GFP-L175G was cytoplasmic (data not shown). As shownin Fig. 9, exogenous expression of MEF2C failed to target thispoint mutant to the nucleus, supporting that direct MEF2 bindingis indeed responsible for nuclear targeting of HDAC4 by MEF2.Along with published reports (20, 41, 43, 61), these resultsindicate that direct binding of 14-3-3 and MEF2 proteins to HDAC4affects its dynamic nucleocytoplasmic shuttling and thereby targetsit to the cytoplasm and the nucleus,respectively.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

HDAC4 is known to function as a transcriptional corepressor (32, 35, 43, 50, 60, 69). Its corepressor functionis subject to regulation by active nucleocytoplasmic trafficking(20, 43, 61). 14-3-3 proteins bind to HDAC4, sequester itto the cytoplasm, and thereby inhibit its corepressor function(20, 61). The results presented herein demonstrate that besidesits 14-3-3 binding sites, HDAC4 possesses additional sequenceelements that are also important for controlling its subcellulardistribution (Fig. 11A).

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FIG. 11. (A) Model depicting how subcellular localization of HDAC4 is controlled. HDAC4 possesses intrinsic nuclear import and export signals important for its dynamic nucleocytoplasmic shuttling. Association with 14-3-3 or MFE2 proteins modulates the shuttling. 14-3-3 binding promotes cytoplasmic localization of HDAC4 by both inhibiting its nuclear import and stimulating its nuclear export, whereas MEF2 interacts with HDAC4 and targets it to the nucleus. While phosphorylation of S246, S467, and S632 of HDAC4 stimulates the binding of 14-3-3 proteins, it remains less clear how the interaction between MEF2 and HDAC4 is regulated. (B) Sequence comparison of the NLS of HDAC4 with the corresponding regions of HDAC5, MITR and HDAC7. Critical residues of the HDAC4 NLS are boxed with related residues of the other three proteins. (C) Sequence alignment of the NES of HDAC4 with the related regions of HDAC5 and HDAC7. Critical residues of the HDAC4 NES are boxed with corresponding residues of HDAC5 and HDAC7.

The N-terminal 118 residues of HDAC4 modulate its nuclear localization. The N-terminal 118 residues play a contributing role in regulating nuclear localization of HDAC4 (Fig. 1). Residues 90 to142 of HDAC4 show limited sequence similarity to MAG1 (Fig. 1A)(7, 63). The distinct subcellular localization between GFP-TM3and -TM4 (Fig. 1) suggests that residues 85 to 105 are importantfor nuclear localization of HDAC4. GFP-TM4 was nuclear in 40 to50% of expressing cells (data not shown); the N-terminal 85 residuesalso modulate subcellular localization ofHDAC4.

How do the N-terminal 118 residues modulate subcellular localization of HDAC4? This region may not be involved in intra- orintermolecular interaction with HDAC4 molecules (Fig. 2). Moreover,neither HDAC1 nor CtBP appeared to modulate subcellular localizationof HDAC4 (data not shown). Although the N-terminal 118 residuesexhibited weak nuclear targeting activity (Fig. 3), this regiondoes not appear to possess a classical arginine-lysine-rich NLS.This region may contain a novel NLS. Alternatively, this regionmay interact with a protein that awaits to beidentified.

In agreement with the latter possibility, a transcriptional repression domain has been mapped to this region (50, 60,69). When tethered, the N-terminal 208 residues of HDAC4 functionas a strong, active transcriptional repression domain. However,neither the N-terminal 118 residues nor residues 118 to 620 areable to repress transcription (60), suggesting that the N-terminal118 residues are necessary but not sufficient for transcriptionalrepression. These findings suggest that this repression domainof HDAC4 may interact with an unidentified nuclear protein. Involvementof the N-terminal 118 residues in such binding may explain therole in modulating subcellular localization of HDAC4. It willbe interesting to identify this elusive protein and study itsrole in regulating subcellular localization and function ofHDAC4.

Tripartite nuclear import signal of HDAC4. Residues 244 to 279 of HDAC4 constitute a functional NLS (Fig. 11A). Mutational analysis of this NLS revealed that three clustersof arginine-lysine residues are necessary for its nuclear importactivity (Fig. 4). Such a tripartite organization is distinctfrom known monopartite or bipartite nuclear import sequences (10,26, 45). It is noteworthy that the HDAC4 mutant 206-326 wasfound to be nuclear, although it still possesses an intact 14-3-3binding site (S246, Fig. 3). Therefore, this NLS is unique andstrong. Since it is arginine-lysine rich, it can be recognizedby importin $alpha$ . Consistent with this, HDAC4 has been found to interactwith importin $alpha$ (20).

Shown in Fig. 11B is the sequence comparison of the HDAC4 NLS with the corresponding regions of HDAC5, MITR, and HDAC7. TheNLS of HDAC4 is highly conserved among these three proteins, suggestingthat their corresponding regions may constitute authentic nuclearimport signals. Consistent with this, an HDAC5 fragment containingthe putative NLS has been very recently shown to possess strongnuclear localization activity (40). Further experiments areneeded to verify the putative import signals of MITR andHDAC7.

Hydrophobic nuclear export signal of HDAC4. Deletion and point mutational analyses revealed that while leucine-rich sequences of HDAC4 do not exhibit nuclear export activity(Fig. 5), a hydrophobic motif (MXXLXVXV) located at its C-terminalend functions as an NES (Fig. 11A). Alanine substitution of thefour critical residue led to nuclear accumulation of the resultingmutants (Fig. 7). These mutants possess all three 14-3-3 bindingsites (20, 61), so they are presumably able to interact with14-3-3 proteins. Therefore, besides the three 14-3-3 binding sites,the NES is also required for cytoplasmic retention ofHDAC4.

This NES is different from most leucine-rich export signals identified in other proteins (45). However, the NES of cyclinB contains only one leucine: LXXXFXXVXI, where X represents anyamino acid residue (39). Although most known export signalsare binding sites of CRM1 (45), CRM1-independent protein nuclearexport pathways have also been found (25, 33). Cytoplasmiclocalization of HDAC4 is sensitive to LMB, a known CRM1-specificinhibitor (14, 30, 46, 51), so CRM1 may be involved inits nuclear export. The nuclear export function of residues 1040to 1069 is LMB sensitive (Fig. 6G), suggesting that CRM1 recognizesthis NES. Consistent with this, we found that HDAC4 and CRM1 functionallyinteract in vivo and that such interaction requires the NES ofHDAC4 (Fig. 8). We also conducted pulldown and coimmunoprecipitationassays to analyze the physical interaction between HDAC4 and CRM1in vitro or in vivo. Various efforts failed to verify this (datanot shown), suggesting that the physical interaction may be transientor too weak to be easilydetected.

Illustrated in Fig. 11C is the sequence comparison of the HDAC4 NES with the corresponding regions of HDAC5 and HDAC7. WhileHDAC7 possesses LXXLXVXI, HDAC5 contains MXXLXVXA. It has beenreported that HDAC5 is mainly nuclear in several cell lines (27,32, 40). We also found that unlike GFP-HDAC4, GFP-HDAC5 wasmainly nuclear in NIH 3T3 cells (data not shown). Interestingly,A1096 of HDAC5 corresponds to V1066 of HDAC4, and the point mutantV1066A of HDAC4 was predominantly nuclear (Fig. 4). Besides thesedistinctions, there are other differences between HDAC4 and HDAC5.First, HDAC5 has been very recently reported to possess an NESwithin the deacetylase domain (40). The corresponding regionof HDAC4 does not appear to be an NES since the mutant 621-1040was pancellular (Fig. 6E). Second, although HDAC4 and HDAC5 arehomologous (overall amino acid sequence identity, 62%; similarity,69%), their sequences are quite divergent in some regions (13,19, 43, 59, 60). Third, unlike S632 of HDAC4, S661 ofHDAC5 does not mediate 14-3-3 binding (20, 41, 61). Finally,while 14-3-3 binding to HDAC4 is constitutive in most cells tested,14-3-3 binding to HDAC5 is dependent on activation of Ca²⁺/calmodulin-dependent kinases (20, 41, 61). Therefore, nuclearexport of HDAC4 and HDAC5 seems to be differentiallyregulated.

Both 14-3-3 and MEF2 proteins regulate intracellular localization of HDAC4. Mapping the NLS and NES of HDAC4 also shed light on how 14-3-3 proteins regulate its subcellular localization. First, theHDAC4 mutant 206-326 was exclusively nuclear, although it hasan intact 14-3-3 binding site (S246, Fig. 3). Second, while mutant315-488 was enriched in the cytoplasm, mutant 315-488/S467A waspancellular (Fig. 5). Third, deletion of residues 1040 to 1084or alanine substitution of the critical residues of the NES ledto nuclear accumulation of the resulting mutants, although thesemutants still contain all three 14-3-3 binding sites (Fig. 6 and7). Finally, the triple mutant TM1 was found to be mainly nuclear(Fig. 1) (20, 61), although its NES remains intact. Takentogether, these findings indicate that both 14-3-3 binding andnuclear export mediated by the NES are required for cytoplasmicretention ofHDAC4.

How does 14-3-3 binding promote cytoplasmic retention of HDAC4? The NLS of HDAC4 is only two residues away from the S246 14-3-3binding site (Fig. 4A), so 14-3-3 binding to S246 may mask theNLS and thereby inhibit its nuclear targeting activity. Consistentwith this, 14-3-3 binding has been found to interfere with theassociation of importin $alpha$ with HDAC4 (20). 14-3-3 binding toS246 of HDAC4 may inhibit access of importin $alpha$ to the NLS. Therefore,one mechanism by which 14-3-3 proteins negatively regulate nuclearlocalization of HDAC4 operates through direct inhibition of importin $alpha$ binding to HDAC4. Substitution of S246 alone was found to beinsufficient to alter cytoplasmic localization of HDAC4 (20,61), so additional mechanisms may be involved. The distinctlocalization of mutants 315-488 and 315-488/S467A (Fig. 5) suggeststhat 14-3-3 binding also stimulates nuclear export of HDAC4. Sinceeach 14-3-3 protein is known to contain an NES (34, 47), bindingof dimeric 14-3-3 proteins to S467 of HDAC4 may provide an activeNES. Therefore, as previously proposed (61), 14-3-3 bindingmay promote cytoplasmic retention of HDAC4 by both inhibitingits nuclear import and stimulating its nuclear export. Similarmodes of action may also apply to some of the other 14-3-3 bindingpartners (16, 44, 64).

Besides 14-3-3 proteins, MEF2 binds to HDAC4 and affects its subcellular localization (Fig. 9) (43). MEF2 was able to directthe mutant 1-208 to the nucleus, although this mutant does notpossess the NLS of HDAC4. Mutational analysis of the MEF2-bindingsite further supports that direct binding of MEF2 promotes nuclearimport of HDAC4. Therefore, HDAC4 possesses multiple sequenceelements controlling its subcellular localization (Fig. 11A). Theintrinsic nuclear import and export signals of HDAC4 dictate itsactive shuttling between the cytoplasm and the nucleus. Such shuttlingleads to a distribution equilibrium. Association of other proteinswith HDAC4 then shifts this equilibrium towards the nucleus orthe cytoplasm. Indeed, direct binding of 14-3-3 and MEF2 proteinsto HDAC4 leads to its cytoplasmic and nuclear localization,respectively.

Cell signaling may regulate HDAC4 through controlling its interaction with 14-3-3 and MEF2 proteins. 14-3-3 binding motifsare putative phosphorylation sites of cyclic AMP- or Ca²⁺-calmodulin-dependent protein kinases, so these kinases may phosphorylateHDAC4, regulate its association with 14-3-3 proteins, and therebyaffect its subcellular localization. Consistent with this, Ca²⁺-calmodulin-dependent kinases have been shown to phosphorylateHDAC5, stimulate binding of 14-3-3 proteins and regulate its nuclearexport (40). Ca²⁺-calmodulin-dependent signaling has also been found to regulateMEF2 binding to HDAC4 (35, 40, 67). Since binding of MEF2to HDAC4 leads to its nuclear localization (Fig. 9) (43), Ca²⁺-calmodulin-dependent signaling may regulate subcellular localizationof HDAC4 through modulating its interaction with MEF2. The recentfinding that oncogenic Ras stimulates localization of HDAC4 tothe nucleus also supports that its subcellular distribution isregulated by cell signaling (70).

In summary, HDAC4 possesses an NLS and an NES for its dynamic shuttling between the cytoplasm and the nucleus. Direct bindingof 14-3-3 and MEF2 proteins alters such shuttling and targetsHDAC4 to the cytoplasm and the nucleus, respectively. The N-terminal118 residues of HDAC4 affect its intracellular localization perhapsthrough interacting with an unidentified nuclear protein. Furtherinvestigation of multiple mechanisms through which cell signalingpathways modulate subcellular localization of HDAC4 shall shedlight on how different deacetylases are differentially regulatedinvivo.

	ACKNOWLEDGMENTS

We thank S. Khochbin and E. N. Olson for sharing results about subcellular localization of HDAC4 and HDAC5, C. M. Grozingerand S. L. Schreiber for HDAC5 expression plasmids, M. Yoshidafor leptomycin B, C. Dargemont and R. Lin for CRM1 cDNA, D. Gorlichfor RanQ69L expression plasmid, J. Han for anti-MEF2C antibody,J. J. LeBrun for use of a FluoChem imaging system, and M. Parkand S. Stifani for use of fluorescence microscopes. A.H.W. isthe recipient of a Canadian Institutes of Health Research (CIHR)doctoral researchaward.

This work was supported by grants from the National Cancer Institute of Canada and a scholarship from the CIHR (to X.-J.Y.).

	FOOTNOTES

^* Corresponding author. Mailing address: Molecular Oncology Group, Royal Victoria Hospital, Room H5.41, McGill University HealthCenter, 687 Pine Ave. West, Montréal, Quebec H3A 1A1, Canada.Phone: (514) 842-1231, ext. 4490. Fax: (514) 843-1478. E-mail:yangxj{at}molonc.mcgill.ca.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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