Epsin 1 Undergoes Nucleocytosolic Shuttling and Its Eps15 Interactor Nh2-Terminal Homology (Enth) Domain, Structurally Similar to Armadillo and Heat Repeats, Interacts with the Transcription Factor Promyelocytic Leukemia Zn2+ Finger Protein (Plzf)

doi:10.1083/jcb.149.3.537

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© The Rockefeller University Press, 0021-9525/2000//537 $5.00
The Journal of Cell Biology, Volume 149, Number 3, , 2000 537-546

Brief Report

Epsin 1 Undergoes Nucleocytosolic Shuttling and Its Eps15 Interactor Nh₂-Terminal Homology (Enth) Domain, Structurally Similar to Armadillo and Heat Repeats, Interacts with the Transcription Factor Promyelocytic Leukemia Zn²+ Finger Protein (Plzf)

Joel Hyman^a^,c, Hong Chen^b^,c, Pier Paolo Di Fiore^d, Pietro De Camilli^b^,c, and Axel T. Brunger^a^,c

^a Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, Connecticut 06520
^b Department of Cell Biology, Yale University, New Haven, Connecticut 06520
^c Howard Hughes Medical Institute, Yale University, New Haven, Connecticut 06520
^d Department of Experimental Oncology, European Institute of Oncology, Milan, Italy
Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, CT 06520.(203) 432-6946(203) 432-6143

brunger{at}laplace.csb.yale.edu

Epsin (Eps15 interactor) is a cytosolic protein involved inclathrin-mediated endocytosis via its direct interactions withclathrin, the clathrin adaptor AP-2, and Eps15. The NH₂-terminalportion of epsin contains a phylogenetically conserved moduleof unknown function, known as the ENTH domain (epsin NH₂-terminalhomology domain). We have now solved the crystal structure ofrat epsin 1 ENTH domain to 1.8 Å resolution. This domainis structurally similar to armadillo and Heat repeats of β-cateninand karyopherin-β, respectively. We have also identifiedand characterized the interaction of epsin 1, via the ENTH domain,with the transcription factor promyelocytic leukemia Zn²+ fingerprotein (PLZF). Leptomycin B, an antifungal antibiotic, whichinhibits the Crm1- dependent nuclear export pathway, inducesan accumulation of epsin 1 in the nucleus. These findings suggestthat epsin 1 may function in a signaling pathway connectingthe endocytic machinery to the regulation of nuclear function.

Key Words: clathrin • Eps15 homology domain • catenin • karyopherin • endocytosis

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Epsin (Eps15 interactor) proteins were recently identified asinteracting partners for the EH (Eps15 homology) domains ofEps15 (Chen et al. 1998; Rosenthal et al. 1999). Both epsin1 and 2 interact with components of the clathrin coat, partiallylocalize at clathrin-coated pits, and are involved in clathrin-mediatedendocytosis (Chen et al. 1998; Rosenthal et al. 1999). The NH₂-terminal140 amino acids of epsin constitute a phylogenetically conservedmodule termed the ENTH domain (epsin NH₂-terminal homology domain;Kay et al. 1999), which is also found in proteins that are substantiallydifferent from epsin outside of this domain (Chen et al. 1998;Kay et al. 1999; Rosenthal et al. 1999). Epsin binding to Eps15(Salcini et al. 1997), as well as to other EH domain-containingproteins (Kay et al. 1999; Hussain et al. 1999; Nakashima et al. 1999;Sengar et al. 1999), is mediated by asparagine-proline-phenylalanine(NPF) motifs, found in the COOH-terminal domain. The centralregion of epsin contains a clathrin binding consensus and multiplecopies of the motif DPW/F typically found in proteins that interactwith the ${alpha}$ -adaptin subunit of the clathrin adaptor AP-2 (Owen et al. 1999;Traub et al. 1999). Accordingly, epsin binds via this regionto both clathrin and AP-2 (Chen et al. 1998; Rosenthal et al. 1999).Epsin 1 is very abundant in brain and probably participatesin membrane recycling at the synapse (Chen et al. 1998).

Yeast homologues of epsin, Ent1p and Ent2p, were shown to beinvolved in endocytosis and actin function (Wendland et al. 1999).The NPF motifs of the Ent proteins bind the EH domains of Pan1,which shares functional similarities with Eps15 (Wendland et al. 1999).Based on genetic studies, the ENTH domain represents the functionallymost important portion of the Ent proteins. Whereas a strainharboring a disruption of both the ENT1 and ENT2 genes is notviable, expression of the ENTH domain of either protein in thisdouble mutant background, but not expression of Entp deletionmutants lacking this domain, was sufficient to rescue the lethalphenotype (Wendland et al. 1999).

So far, the function of the ENTH domain is unknown. To gaininsight into its function, we have determined the X-ray crystalstructure of the ENTH domain of rat epsin 1 and investigatedits protein-binding properties. Our findings suggest an unexpecteddual function of epsin in the cytoplasm and in the nucleus.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

ENTH Expression for Structural Determination
ENTH of rat epsin 1 was expressed as an NH₂-terminal GST fusionusing the pGEX-6-1 expression vector (Amersham Pharmacia Biotech).The plasmid was introduced into B834(DE3) cells (Novagen) andgrown in defined M9 media supplemented with 50 mg/liter selenomethionine(SeMet; Leahy et al. 1994) and 0.1 mg/ml ampicillin. Cells weregrown to an optical density of 2 measured at 600 nm, at whichtime the culture was induced using 0.8 mM isopropyl-B-D-thiogalactopyranosideand allowed to continue growing for $~$ 4–5 h. Cells wereharvested by centrifugation, flash frozen, and stored at –80°C.Protein purification was performed using 60 g of frozen cellsresuspended in 200 ml of 50 mM Tris-HCL, pH 7.5, 200 mM NaCl,10 mM DTT, and 2 mM PMSF, and were then homogenized by sonification.The cell lysate was pelleted by centrifugation at 46,000 g and4°C for 50 min. The supernatant was added to 3 ml of glutathioneSepharose 4B beads (Amersham Pharmacia Biotech). After gentlemixing for 1 h, GST-Sepharose beads containing bound ENTH werewashed four times with 50 ml wash buffer (20 mM Tris-HCl, pH7.5, 200 mM NaCl, and 10 mM DTT). GST-Sepharose beads with boundENTH were then resuspended in 15 ml of wash buffer with $~$ 100µg bovine thrombin and incubated overnight with agitation.As a note, although pGEX6-1 is a rTEV cleavable GST fusion vector,we found that rTEV cleavage was not effective. However, thrombincleaves quite well at an internal site 10 amino acids into theENTH domain. Crystals of lesser quality have been obtained withrTEV cleaved protein, but this protein showed significant degradationin crystal trays, so studies with these crystals were not pursued.Cleaved ENTH protein was separated from glutathione-Sepharosebeads and injected onto a Superdex 75 16/60 size-exclusion column(Amersham Pharmacia Biotech) at 0.5 ml/min in wash buffer. Fractionscontaining ENTH as determined by UV absorption and SDS-PAGEwere pooled and dialyzed into 20 mM Na-Hepes, pH 7.5, 20 mMNaCl, and 10 mM DTT. ENTH was then concentrated to $~$ 7.5 mg/ml(Millipore ultrafree spin concentrator), flash frozen in 100µl aliquots using liquid nitrogen, and stored at –80°C.

Crystallization and Data Collection
Initial crystals were obtained by hanging drop vapor diffusionat 20°C. 1 µl of protein solution at $~$ 7.5 mg/ml wasmixed with 1 µl of mother liquor containing 100 mM Na-Hepes,pH 7.5, 10% polyethylene-glycol (PEG) 1000, and 8% ethyleneglycol on a siliconized glass coverslip, and equilibrated against0.5 ml of mother liquor. Crystals typically grew to full size(220 x 220 x 100 µm) in 30–40 h. Crystals were cryoprotectedby sequential transfer into mother liquor containing 5% increasingincrements of ethylene glycol to a final concentration of 30%.The crystals were then flash frozen in liquid nitrogen-cooledliquid propane that was subsequently frozen in liquid nitrogen.ENTH crystallized in space group P3₁21 with one molecule perasymmetric unit, and a solvent content of 40% as determinedby the Matthews coefficient (Matthews 1968). Diffraction datawere collected at four wavelengths, and processed using DENZO/scalepack(Otwinowski and Minor 1997; Table ).

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Table 1 Crystallographic Data Collection Statistics

Structure Determination
Four of the five expected selenium sites were located in ananomalous difference Patterson map calculated at the peak wavelengthusing an automated Patterson heavy-atom search method (Grosse-Kunstleveand Brunger, 1999) implemented in the Crystallography &NMR System (CNS; Brunger et al. 1998). The final site was locatedafter initial multiwavelength anomalous dispersion (MAD) phasingwith CNS using a log likelihood gradient map (Bricogne 1997).The MAD phasing statistics were excellent (Table ). The phaseswere improved by density modification using solvent flipping(Abrahams and Leslie 1996) and histogram matching (Zhang and Main 1990;Table ). A representative region of the resulting electron densitymap is shown in Fig. 1. Nearly all side chains were clearlydefined in the electron density map. All map and phasing calculationswere carried out using CNS (Brunger et al. 1998).

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Table 2 Crystallographic Phasing Statistics

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Table 3 Crystallographic Figure-of-Merit

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Figure 1 Representative experimental electron density map for residues 30–44, 72–76, and 81–85 contoured at 1.4 Å obtained by MAD phasing and subsequent density modification. The final refined model is shown using a ball and stick representation, with residues in yellow indicating a high degree of sequence conservation. The backbone trace was clearly visible for a portion of ${alpha}$ helix 2, and exceptional density was found for most side chains. Figure generated using MOLSCRIPT (Kraulis 1991).

Model Building and Refinement
An initial model was built with the program O (Jones et al. 1991),using the electron density map obtained by MAD phasing and subsequentdensity modification. All of the ENTH domain could be unambiguouslytraced except for residues 1–5, 20–23, 149, and150. Model refinement was monitored using the free R value (Brunger 1992)computed from a randomly omitted 10% of the observed diffractiondata. Refinement was carried out using alternating rounds ofsimulated annealing, torsion angle molecular dynamics (Riceand Brunger, 1994), restrained B factor refinement (Hendrickson 1985),and model rebuilding. Model refinement was accomplished in CNSusing the MLHL target (Pannu and Read 1998) against the diffractiondata at the low-energy remote wavelength. Final model statisticsare given in Table and were calculated using CNS (Brunger et al. 1998)and Denzo (Otwinowski and Minor 1997). The final model containsresidues 16–160 of the ENTH domain, 65 ordered water molecules,and 3 ethylene glycol molecules.

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Table 4 Crystallographic Refinement

Yeast Two-hybrid Screen
The ENTH domain of rat epsin 1 (amino acids 1–160 of ratepsin 1; Chen et al. 1998) fused to the LexA DNA-binding domainwas used as bait to screen a rat brain Matchmaker activationdomain library in pGAD10 (CLONTECH Laboratories, Inc.). Thebait was transformed along with the library in the L40 reporteryeast strain. Yeast colonies that survived on histidine–plates were also tested for activation of the LacZ gene. Preyplasmids positive for LacZ were retransformed in yeast. Clonesthat did not transactivate with the LexA DNA-binding vectoralone, but interacted with the ENTH-LexA DNA-binding domain,were restriction mapped and sequenced. A pair of primers specificto pGAD10 vector: 5' CAT TTC GAT GAT GAA GAT ACC CCA CCA AACC 3', 5' GTG CAC GAT GCA CAG TTG AAG TGA ACT TGC 3'; were usedfor PCR of the inserts that were subjected to restriction mappingand sequence analysis. The specificity of the interaction betweenrPLZF ${Delta}$ POZ (see Results) with the ENTH domain was further confirmedby testing the interaction of rPLZF ${Delta}$ POZ-LexA DNA-binding domainwith ENTH-Gal4 activation domain in the yeast two-hybrid assay.Deletion mutants of rPLZF ${Delta}$ POZ were generated by PCR amplificationof the desired fragments, which were subcloned into the pGAD424activation domain vector (CLONTECH Laboratories, Inc.).

Affinity Purification
For affinity-purification of rat brain proteins, the same ENTHdomain used for crystallographic studies was coupled to UltraLinkBiosupport Medium (Pierce Chemical Co.) according to the manufacturer'sinstructions. A Triton X-100 extract of a rat brain total homogenate(10 mg/ml) was incubated with immobilized ENTH domain at 4°Cand the bound material was analyzed by SDS-PAGE and Westernblotting. Wild-type and mutant GST-ENTH fusion proteins wereused for affinity purifications from Triton X-100 extracts ofcells transfected with flag epitope-tagged rPLZF ${Delta}$ POZ or full-lengthhuman promyelocytic leukemia Zn²+ finger protein (PLZF) accordingto standard procedures (Nemoto et al. 1997).

Generation of Mutant ENTH Domains
The mutant ENTH domains were obtained using PCR-based site-directedmutagenesis (Chen et al. 1999). The sequences of these mutantENTH domains were confirmed by standard double-strand sequencing.

Leptomycin B Incubations
Leptomycin B (10 ng/ml; kind gift of Dr. M. Yoshida; Kudo et al. 1999)was added to the culture medium 16 h after transfection andcells were incubated for additional 3.5 h before fixation. Afull-length GFP-tagged rat epsin 1 clone was constructed asdescribed (Rosenthal et al. 1999) and used in the leptomycinB studies.

Antibodies and Miscellaneous cDNAs
Rabbit polyclonal antibodies against human PLZF and epsin werepreviously described (Chen et al. 1998; Grignani et al. 1998).Rabbit polyclonal antibodies against rat PLZF were obtainedusing GST-rPLZF ${Delta}$ POZ as the immunogen. The resulting serum wasfirst depleted of anti-GST antibodies by incubation with GSTbeads and then affinity-purified with GST-rPLZF ${Delta}$ POZ fusion protein.A cDNA encoding GFP-β-galactosidase fusion protein in pHM830was a kind gift of Dr. T. Stamminger (Institute fur Klinischeund Molekulare Uirologie, Universitat Erlangen-Nurnberg, Erlangen,Germany). Xpress-tagged epsin 1 cDNA was previously described(Chen et al. 1998). A human PLZF cDNA in pcDNA3 was a kind giftof Dr. P.G. Pelicci (European Institute of Oncology, Milano,Italy). The cDNA encoding GFP-rat epsin 1 was generated by subcloningthe epsin 1 cDNA into the pEGFP-C1 vector (CLONTECH Laboratories,Inc.).

Miscellaneous Procedures
Cell transfection, immunoprecipitation, immunofluorescence,GST-fusion protein production, SDS-PAGE, Western blotting, andprotein assay were carried out as previously described (Chen et al. 1998).

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Structure Determination
The ENTH domain of rat epsin 1 (residues 1–160) was expressedas a GST-fusion protein in Escherichia coli. After cleavageof the fusion protein and purification, crystals of the ENTHdomain were obtained by hanging drop vapor diffusion in a polyethylene-glycolcondition at 4°C. SeMet-substituted ENTH domain crystallizedin a similar condition, and these crystals were used for furtherstudy. Diffraction data were collected for a MAD experiment(Hendrickson 1991) using synchrotron radiation at four wavelengthsaround the selenium K absorption edge. Crystals belonged tospace group p3₁21, with unit cell parameters: a = b = 49.81Å, c = 99.97 Å, ${alpha}$ = β = 90°, and ${gamma}$ = 120°.The crystals contained $~$ 40% solvent and diffracted to a minimumBragg spacing of 1.8 Å. The electron density map obtainedfrom density-modified MAD phases was superb, and easily traceable(Fig. 1). The final refined model has a free R value (Brunger 1992)of 22.5% for all reflections with a Bragg spacing >1.8 Å.

General Features of the Structure
The ENTH domain forms a compact globular domain (Fig. 2A andFig. B) with a solvent accessible surface area of $~$ 8,200 Å.The structure is composed of eight ${alpha}$ helices connected by loopsof varying length. The general topology of the structure isdetermined by three helical hairpins ( ${alpha}$ 1–2, ${alpha}$ 3–4,and ${alpha}$ 6–7) that are stacked consecutively with a right-handedtwist. This stacking gives the ENTH domain a rectangular appearancewhen viewed face on (Fig. 2A i and B i). The two primary faces,one concave and one convex, are made up of parallel ${alpha}$ helices(Fig. 2 A). The COOH-terminal ${alpha}$ helix ( ${alpha}$ 8) folds back across thedomain, framing the bottom edge perpendicular to the centralhairpin ( ${alpha}$ 3–4). From the opposite edge, loops that connect ${alpha}$ helices 1–2, 3–4, and 6–7 form a conicalprojection, lending a wedge-like appearance (Fig. 2A i).

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Figure 2 Overall structure of the ENTH domain and sequence alignment. A, Ribbon drawings of the ENTH domain. The drawing at right (ii) is related to the drawing at left (i) by a 60° rotation towards the viewer. The eight ${alpha}$ helices of the ENTH domain are indicated by different colors. The T28A, R72A, and G88S mutations made in this study are indicated by aquamarine balls. ${alpha}$ Helices 1–8 are indicated in i. Figures generated using MOLSCRIPT (Kraulis 1991). B, Sequence conservation projected onto accessible surface representations of the ENTH domain. These surface representations correspond to the same two views (i and ii) in A. Figures generated using GRASP (Nicholls, 1991). C, Sequence alignment of ENTH domains from various species. Identical residues are indicated in red, conserved residues in yellow. Green stars indicate residues that have been mutated in this study. The schematic diagram above the alignment indicates the location of loop and helix regions. Accession number and species as follows: epsin 1, AAC33823, Rattus norvegicus; epsin 2b, AAC78609, Homo sapiens; BAA11488, Homo sapiens; MP90, AAC60123, Xenopus laevis; liquid facets, AAF05113, Drosophila melanogaster; Ent1, 6320039, S. cerevisiae; Ent2, 6323235, S. cerevisiae; 6322585, S. cerevisiae; AAC64305, Arabidopsis thaliana; CAA19587, Schizosaccharomyces pombe; AF-10, AAB68030, Avena fatua. Alignment generated using CLUSTAL W (Thompson et al. 1994) and AMAS (Livingston and Barton 1993).

The ENTH domain family contains several highly conserved residues(Chen et al. 1998; Kay et al. 1999; Rosenthal et al. 1999; Fig. 2C). The most highly conserved residues fall roughly into twoclasses: internal residues that are involved in packing andtherefore are necessary for structural integrity, and solventaccessible residues that may be involved in protein–proteininteractions. Two large regions of high conservation emergeon the molecular surface: a larger patch formed primarily fromresidues on loop 2 and ${alpha}$ helix ${alpha}$ 4, and a smaller patch was foundnear loop 7 (Fig. 2A, Fig. B, and Fig. C).

Structural Alignment and Comparison
A structural similarity search using DALI (Holm and Sander 1993)identified proteins that are structurally similar to ENTH, butnot related by primary sequence. The ENTH structure is mostsimilar to an armadillo repeat segment from β-catenin (Huber et al. 1997;Fig. 3A and Fig. B), the HEAT repeat unit from karyopherin-β(importin-β; Chook and Blobel 1999; Cingolini et al. 1999;Fig. 3C and Fig. D), and to the scaffolding subunit of proteinphosphatase 2A (Groves et al. 1999). Both armadillo and HEATrepeats are protein–protein interaction modules composedexclusively of ${alpha}$ helices, and form structures with two primaryfaces, one concave and one convex. armadillo and HEAT repeatsbind to target proteins with their concave face (Huber et al. 1997;Chook and Blobel 1999; Cingolini et al. 1999; Groves et al. 1999).Structural superimposition of the ENTH domain with either typeof repeat aligns their concave faces (Fig. 2 and Fig. 3), whichcontain the largest patch of conserved surface residues (Vriend 1990).The C superposition of ENTH with karyopherin-β has a rootmean square difference (RMSD) of 1.5 Å, whereas the Csuperposition with β-catenin produces an RMSD of 1.8 Å.

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Figure 3 Alignment of structurally similar protein folds. A, Alignment of the ENTH domain of epsin 1 (blue) with one portion of the armadillo repeat region of β-catenin (green), showing a good overall superimposition between ${alpha}$ helices in the central region of the domain. This alignment shows the ENTH domain in the same orientation as in Fig. 2A ii. B, Same as A, but showing the entire β-catenin armadillo region and the ENTH domain in the same orientation as in Fig. 2A i. C, Alignment of the ENTH domain (blue) with a segment of karyopherin-β (orange). This alignment shows the ENTH domain in the same orientation as in Fig. 2A ii. D, Same as C, showing the entire structure of karyopherin-β and the ENTH domain in the orientation of Fig. 2A i. Structural alignments produced using WHATIF (Vriend 1990). Figures generated using MOLSCRIPT (Kraulis et al., 1991).

Isolation of an ENTH Domain Binding Protein, PLZF
The structural similarity of the ENTH domain to armadillo andHEAT repeats suggests that the ENTH domain may interact withother proteins. We searched for potential binding partners ofthe ENTH domain of rat epsin 1 (residues 1–160) usingthe yeast two-hybrid method. A bait construct consisting ofthe ENTH domain fused to the DNA-binding domain of LexA wasused to screen a pGAD10 rat brain cDNA library. 20 of the clonesisolated by the screen were all identical, and encoded an openreading frame highly homologous (96% identity) to the COOH-terminalportion of human PLZF (corresponding to amino acids 262–673of the human protein). PLZF is a transcription factor containingan NH₂-terminal BTB/POZ domain and nine C₂H₂ Zn²⁺ finger motifs(Li et al. 1997; Fig. 4 A).

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Figure 4 Interaction between the ENTH domain of epsin 1 and PLZF. A, Schematic representation of human PLZF and of the rat PLZF fragments discussed in this study. Numbers indicate amino acid numbers. B, Interaction of the GST-ENTH domain fusion protein with rPLZF ${Delta}$ POZ. An extract of CHO cells transfected with flag-tagged rPLZF ${Delta}$ POZ was affinity-purified on either GST or a GST-ENTH domain fusion protein. The starting material and the bead-bound material were analyzed by Western blotting using antibody directed against the flag epitope. C, ENTH domain affinity purification from a rat brain extract. A Triton X-100 extract of a rat brain total homogenate was affinity-purified on ENTH domain conjugated to beads or control beads. The starting material and the bead-bound material were analyzed by Western blotting for PLZF. D and E, PLZF and epsin can be coprecipitated from a rat brain Triton X-100 extract. D, Immuno-precipitates generated by antiepsin 1 antibodies or control IgGs were analyzed by Western blotting with anti-rat PLZF or anti-p53 (used as control) antibodies. E, Immunoprecipitates generated by anti-PLZF antibodies or control IgGs were analyzed by Western blotting using antiepsin 1 antibodies. F: Mutant ENTH domains fail to interact with PLZF. An extract of CHO cells transfected with flag-tagged human PLZF was affinity-purified on wild-type or mutant (T28A, R72A, and G88S) GST-ENTH domain fusion proteins. The starting material, the bead-unbound and the bead-bound material were analyzed by Western blotting using antibody directed against the flag epitope or anticlathrin antibody as a control. B, Bead-bound; c, control IgGs; e, antiepsin antibodies; P, pellet; S, supernatant; SM, starting material; U, bead-unbound.

The identification of a transcription factor as an interactionpartner for the ENTH domain of epsin 1 seemed surprising atfirst, given the known function of epsin 1 at the cell periphery.However, β-catenin family proteins, which contain a structurallyrelated module, have a dual function in the cell cortex andin the nucleus (Barth et al. 1997; Willert and Nusse 1998).Furthermore, catenin p120, which contains armadillo repeats,binds to a POZ/BTB-Zn²⁺ finger containing transcription factor,Kaiso, that is homologous to PLZF (Daniel and Reynolds 1999).The interaction of catenin p120 with Kaiso is mediated by thearmadillo repeat region of p120, and by the COOH-terminal portionof Kaiso, corresponding to the region of PLZF selected by theyeast two-hybrid screen. In addition, based on the binding propertiesof protein fragments, the Zn²⁺ finger region and upstream sequencesof both Kaiso and PLZF are required for the interaction withcatenin p120 and ENTH, respectively (Daniel and Reynolds 1999;and Fig. 4 A). The similarity of these two interactions is likelyto reflect evolutionary conservation. We hypothesized that epsinand PLZF are physiological partners, and carried out furtherbiochemical and functional studies to validate this interaction.

Biochemical Interaction of Epsin and PLZF
To verify the interaction of PLZF and epsin, affinity purificationexperiments were performed using immobilized ENTH domain. TheGST-ENTH domain, but not GST alone, specifically retained aflag-tagged–rPLZF ${Delta}$ POZ fragment (the protein fragment ofPLZF lacking the POZ domain, corresponding to the fragment isolatedby the yeast two-hybrid screen) from extract of transfectedCHO cells (Fig. 4 B). In addition, purified GST-free ENTH domainconjugated to beads, but not beads alone, interacted with endogenousPLZF from a rat brain extract (Fig. 4 C).

To determine whether epsin and PLZF interact in vivo, immunoprecipitationexperiments from rat brain extracts were carried out. Antiepsinantibody, but not control IgGs, coprecipitated PLZF, but notp53 (a negative control; Fig. 4 D). Conversely, anti-PLZF antibody,but not preimmune IgGs, coprecipitated epsin (Fig. 4 E), butnot p53 (not shown). While epsin is present in the cytosol andfurther concentrated at the synapse, PLZF was shown to be primarilylocalized in the nucleus (Ruthardt et al. 1998). However, acytosolic pool of PLZF was observed by immunofluorescence inbrain (not shown).

To further assess the specificity of the binding of the ENTHdomain to PLZF, highly conserved residues of the ENTH domainwere altered by site directed mutagenesis: T28 to A, R72 toA, and G88 to S. Mutation of glycine at position 88 was previouslyfound to confer temperature sensitivity to the function of yeastEnt1p (Wendland et al. 1999). Wild-type and mutant ENTH domainswere expressed as GST fusion proteins and used to affinity purifyflag-tagged human PLZF expressed in CHO cells. As shown by Fig. 4F, wild-type, but not mutant ENTH domains, pulled down PLZFfrom transfected cell extracts. A control protein, clathrin,was not retained by any of these fusion proteins.

PLZF Can Recruit Epsin to the Nucleus
Based on immunofluorescence, most epsin is found in the cytosol,even after overexpression (Chen et al. 1998; Rosenthal et al. 1999;Fig. 5 A). The interaction of epsin 1 with PLZF raises the possibilitythat epsin may be found in the nucleus under certain conditions.Enhanced expression of PLZF may increase the fraction of epsin1 localized in the nucleus and allow the visualization of anuclear epsin pool by immunofluorescence. When either full-lengthhuman PLZF or rPLZF ${Delta}$ POZ were overexpressed by transfection, bothproteins partially accumulated in the nucleus (Fig. 5 A, andnot shown). In cells cotransfected with epsin 1 and PLZF, anuclear pool of epsin was also observed (the concentration ofendogenous epsin is below detectability with our antibodies;Chen et al. 1998).

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Figure 5 Immunofluorescence micrographs demonstrating that epsin may accumulate in the nucleus. A, Overexpression of human PLZF induces a partial accumulation of epsin in the nucleus. CHO cells were transiently transfected with epsin alone, human PLZF alone, or both proteins together, and then analyzed by confocal microscopy immunofluorescence. A pool of epsin is localized in the nucleus only in cells expressing both proteins. B, Leptomycin B induces an accumulation of epsin in the nucleus. CHO cells were transiently transfected with GFP-epsin, Xpress-tagged epsin, or the control protein GFP-β-galactosidase (GFP-βgal) and incubated for 3.5 h in the presence of leptomycin B before microscopic analysis. An accumulation of epsin is observed in the nucleus only in cells treated with leptomycin B. GFP-β-galactosidase was only cytosolic both in the presence and in the absence of leptomycin B. Bars, 12 µm.

We next investigated whether epsin physiologically shuttlesbetween the nucleus and the cytoplasm. The antifungal antibiotic,leptomycin B, was recently shown to block the Crm1-dependentnuclear export pathway and to induce a nuclear accumulationof several proteins which shuttle between the nucleus and thecytoplasm (Nishi et al. 1994; Kudo et al. 1999; Van Hengel et al. 1999).We examined whether leptomycin B affected the intracellulardistribution of epsin in CHO cells transiently transfected witheither GFP-epsin 1 or Xpress-tagged epsin 1. As shown by Fig. 5B, both epsin 1 fusion proteins accumulated in the nucleus afterincubation with leptomycin B, but not in control cells. A GFP–β-galactosidasefusion protein used as a control did not accumulate in the nucleusregardless of the presence of leptomycin B.

Discussion

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

The crystal structure of the ENTH domain of epsin 1 revealeda relationship to other well characterized protein modules thatcould not have been predicted by primary amino acid sequenceanalysis. The ENTH domain adopts a fold strikingly similar tothat of armadillo and HEAT repeats, two domains found in β-cateninand karyopherin, respectively. Structural similarity often indicatesfunctional similarity. Accordingly, we have identified propertiesof epsin suggesting that this similarity is functionally meaningful.

β-Catenin was first discovered as a component of a cytoskeletalscaffold underlying the plasma membrane and is thought to playan important role in the function of the cortical cytoskeleton(Tao et al. 1996; Bullions and Levine 1998). β-Cateninwas subsequently found to be part of a signaling pathway fromthe cell surface to the nucleus, the so-called Wnt signalingpathway. Activation of the pathway leads to decreased phosphorylationand degradation of β-catenin and to its accumulation inthe nucleus, where it regulates transcription (Barth et al. 1997;Willert and Nusse 1998; Peifer and Polakis 2000). Mammalianepsin was identified as an accessory factor in clathrin-mediatedendocytosis (Chen et al. 1998; Kay et al. 1999; Rosenthal et al. 1999)and its homologues in yeast, Ent1p and Ent2p, were implicatedboth in endocytosis and actin function (Wendland et al. 1999).The predominant pool of epsin is localized in the cytosol (Chen et al. 1998;Rosenthal et al. 1999). However, our present results demonstratethat epsin binds a transcription factor, PLZF, and that it canenter the nucleus. More specifically, the nuclear accumulationof epsin produced by leptomycin B demonstrates that epsin shuttlesphysiologically between the cytoplasm and the nucleus. LeptomycinB blocks the Crm1-dependent nucleocytosolic export pathway (Nishi et al. 1994;Kudo et al. 1999; Van Hengel et al. 1999), thus implying thatnuclear accumulation of epsin results from an imbalance betweennuclear import and nuclear export. An attractive possibilityis that a regulated interaction of epsin with cytosolic components,possibly mediated by its phosphorylation (Chen et al. 1999),may control the nuclear pool of epsin and, via PLZF, the transcriptionof specific genes. This regulation may occur in response toexternal stimuli that activates endocytosis. This scenario definesa new regulatory pathway from the endocytic machinery to thenucleus.

These findings are convergent with recent studies of the epsinbinding protein Eps15. As in the case of epsin, the role ofEps15 in clathrin-mediated endocytosis is well established andthe bulk of Eps15 is localized in the cytosol (Salcini et al. 1997;Benmerah et al. 1998). However, an additional role of Eps15in the regulation of nuclear functions has emerged. The sameEH domain containing region of Eps15 that binds epsin also interactswith Numb and RAB/Hrb (Salcini et al. 1997). Numb binds Mdm2,a negative regulator of p53 (Juven-Gershon et al. 1998; Juven-Gershon and Oren 1999),demonstrating a connection between Eps15 and a transcriptionfactor. RAB/Hrb is a cofactor for export from the nucleus ofthe HIV protein Rev, and the EH domains of Eps15 cooperateswith RAB/Hrb in the function of the Rev export pathway (Doria et al. 1999).This export pathway, in turn, is Crm1-dependent (Ullman et al. 1997).The role of Eps15 as a cofactor in nucleocytosolic export raisesthe possibility that even the similarity of the ENTH domainof epsin to the karyopherins may reflect some functional relationship.The karyopherins are proteins implicated in cargo transportand recognition across the nuclear envelope via their HEAT repeatdomains (Radu et al. 1995; Görlich 1998; Pemberton et al. 1998;Nakielny and Dreyfuss 1999).

Based on genetic studies, the ENTH domain is the most importantfunctional domain of the yeast epsins, Ent1p and Ent2p (Wendland et al. 1999).Since the residues of the Ent proteins that interact with yeastEH domains and clathrin are localized outside the ENTH domain,the essential role of this domain may reflect its implicationin nuclear functions. This possibility is consistent with ourobservation that at least one of the residues important forthe function the ENTH domain of Ent1p is also required for thebinding of rat epsin 1 ENTH domain to PLZF. Although an obviousorthologue of PLZF is not present in Saccharomyces cerevisiae,proteins with multiple Zn²⁺ finger motifs similar to those ofPLZF are expressed by this organism. The similarity of PLZFto Kaiso, another transcription factor previously shown to bindthe armadillo repeat region of catenin p120 (Daniel and Reynolds 1999),indicates that the interaction of armadillo-repeat domains withthis family of transcription factors is evolutionary conserved,and therefore likely to be physiologically important. The interactionof the ENTH domain with a transcription factor is not mutuallyexclusive with potential interactions with other proteins. Basedon the property of the structurally related armadillo and HEATrepeats to bind multiple partners (Barth et al. 1997; Huber et al. 1997;Willert and Nusse 1998; Chook and Blobel 1999; Cingolini et al. 1999;Groves et al. 1999), it is likely that even the ENTH domainmay have multiple physiological interactors. Pull-down experimentsfrom rat brain have shown that tubulin, and to a lower extentcoatomer (Rothman and Wieland 1996), can bind ENTH domain ofepsin 1 (our unpublished observations). However, the possiblesignificance of these interactions remains unclear.

ENTH domains are present not only in proteins of the epsin family,but also in proteins which differ substantially from epsin outsidethis domain (Chen et al. 1998; Kay et al. 1999; Rosenthal et al. 1999).It is of interest that certain motifs are frequently found insuch proteins. Besides NPF motifs that bind EH domains (Salcini et al. 1997),AP-2 and clathrin motifs, as well as FG motifs, are often presentin them (Kay et al. 1999). FG repeats are signature motifs ofnucleoporins (Radu et al. 1995), further emphasizing a potentialconnection of the ENTH domain to nuclear function. While epsin1 does not contain FG repeats, most other epsin family membersdo (three or more such repeats are present in yeast Ent1 andEnt 2, in mammalian epsin 2, and in the epsin-like protein D79993.1).It is therefore possible that a dual function at the cell surfaceand in the nucleus may be a general property of most, possiblyall, ENTH containing proteins.

Acknowledgments

We thank Dr. M. Yoshida (University of Tokyo, Tokyo, Japan)for the kind gift of leptomycin B; Dr. E. Coutavas (RockefellerUniversity, NY) for suggestions; C. Stroupe, M. Wilson, andH. Bellamy for help during data collection at SSRL BL1-5 (theSSRL Biotechnology Program is supported by the National Institutesof Health, National Center for Research Resources, BiomedicalTechnology Program, and by the Department of Energy, Officeof Biological and Environmental Research); L. Rice and P. Adamsfor discussions and advice concerning model building and refinement;Brunger Lab members for critical reading of the manuscript;P.G. Pelicci, A. Zelent (London, UK), and T. Stamminger forthe gift of reagents, and the Yale Biotechnology Keck facilityfor DNA analysis.

This work was supported in part by grants from the NationalInstitutes of Health (CA46128 and NS36252) to P. De Camilli.

Note Added in Proof. Mao et al. (Mao, Y., A. Nickitenko, X.Duan, T.E. Lloyd, N.N. Wu, H. Bellen, and F.A. Quiocho. 2000.Cell. 100:447–456) have recently reported the structureof VHS and FYVE tandem domains from the hepatocyte growth factor-regulatedtyrosine kinase substrate. The VHS and ENTH domains align withan RMSD of $~$ 1.8 Å, indicating an extremely similar fold.This is especially interesting because HRS is involved in membranetrafficking and signal transduction, perhaps indicating thatthis fold is a common motif in these areas.

Submitted: 28 January 2000

Revised: 17 March 2000

Accepted: 17 March 2000

Joel Hyman and Hong Chen contributed equally to this work.

The coordinates and structure factors have been deposited withthe Research Collaboratory for Structural Bioinformatics (RSCB),accession number 1edu, and will also be available at http://atb.csb.yale.edu

Abbreviations used in this paper: CNS, Crystallography &NMR System; EH, Eps15 homology; ENTH domain, epsin NH₂-terminalhomology domain; epsin, Eps15 interactor; MAD, multiwavelengthanomalous dispersion; NPF motifs, asparagine-proline-phenylalaninemotifs; PLZF, promyelocytic leukemia Zn²+ finger protein; RMSD,root mean square difference; SeMet, selenomethionine.

References

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Abstract
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References

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