From the Section of Biochemistry, Molecular and Cell Biology, Cornell University, Ithaca, New York 14853
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ABSTRACT |
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EBP50 (ezrin-radixin-moesin-binding phosphoprotein 50) was recently identified by affinity chromatography on the immobilized NH2-terminal domain of ezrin. Here we map and characterize the regions in EBP50 and ezrin necessary for this association. Using blot overlays and in solution binding assays, the COOH-terminal 30 residues of EBP50 were found to be sufficient for an association with residues 1-286 of ezrin. EBP50 did not bind to full-length (1-585) ezrin, indicating that the EBP50 binding site is masked in the full-length molecule. Ezrin contains two complementary self-association domains known as N- and C-ERMADs (ezrin-radixin-moesin-association domains), encompassing residues 1-296 and 479-585, respectively. An ezrin 1-583 construct lacking the two terminal residues necessary for this association was found to have an unmasked EBP50 binding site. Moreover, binding of EBP50 and the C-ERMAD to ezrin residues 1-296 was found to be mutually exclusive, with the C-ERMAD having a higher affinity. These results suggest that in full-length ezrin, the binding site for EBP50 is masked through an intramolecular N/C-ERMAD association. Based on these and additional results, we propose a model whereby dormant ezrin can be activated to bind EBP50 on its NH2-terminal end and F-actin on its COOH-terminal end. Since EBP50 is proposed to bind membrane proteins through its PDZ domains, this provides a molecular description of the regulated linkage of microfilaments to membranes in cell surface microvilli.
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INTRODUCTION |
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Polarized epithelial cells assemble distinct apical and
basolateral domains for the transport of small molecules. The apical domain is generally characterized by the presence of abundant microvilli in which reside specific membrane-bound transport proteins. Recent studies aimed at understanding the mechanism of microvillus formation have focused on ezrin, a member of the ezrin-radixin-moesin (ERM)1 protein family that
performs both a regulatory and structural role in the assembly of
microvilli (1-3). The ERM proteins show ~75% overall sequence
identity to each other and are related through their
NH2-terminal domain residues to band 4.1, a membrane
cytoskeletal-linking protein of the erythrocyte (4-7). Another member
of the band 4.1 superfamily is merlin, the product of the
neurofibromatosis 2 tumor suppressor gene, which shares about 60%
identity to ERM proteins over this same region (8, 9). The ERM
proteins, which are about 580 residues in length, have a ~300 residue
NH2-terminal domain that can interact with the cytoplasmic
domain of the transmembrane protein CD44 (10), the PDZ
domain-containing ERM-binding phosphoprotein 50 (EBP50) (11, 12), or
the Rho-GDP dissociation inhibitor (Rho-GDI) (13). Following this
domain is a region predicted to be largely -helical. An F-actin
binding site has been mapped to the 34 COOH-terminal residues (14, 15),
although recent studies suggest that association with actin might be
more complex (16).
In addition to these potential interactions, the ERM proteins have the ability to form homo- and heterotypic associations between family members (17). The first 296 residues of each member defines a domain that can form a high affinity association with the 107-residue COOH-terminal region of any ERM protein; these have been called NH2- and COOH-ERM association domains (N- and C-ERMADs) (18). These self-association domains are not constitutively available for spontaneous oligomerization in vivo, as the bulk of ezrin exists in the cytoplasm in a monomeric form (19, 20). Studies with native monomeric ezrin have revealed that the C-ERMAD, as well as the COOH-terminal F-actin binding site, is conformationally masked (18). Regulated self-association seems to be physiologically relevant as dimers and other oligomers are the predominant forms of ezrin in isolated placental microvilli, and dimer formation can be induced in cultured cells by the activation of signaling pathways in a time course that parallels microvillus assembly (21). These combined results led us to propose that the bulk of the ezrin in cells exists in a dormant monomeric conformation in which sites for self-association and association with other proteins are masked. Ezrin activation is proposed to lead to the exposure of sites for both oligomerization and interaction with membrane and cytoskeletal components (21, 1).
We recently described human EBP50, a 358-residue protein that was identified by affinity chromatography on resins containing the NH2-terminal domains of ezrin or moesin (11). Analysis of the EBP50 sequence revealed that it contains two PDZ domains followed by a ~120-residue COOH-terminal tail. Localization of EBP50 in tissues and cultured cells shows that it colocalizes with ezrin in apical microvilli. The existence of complexes of ezrin and EBP50 in extracts of isolated microvilli indicates that the binding of EBP50 to ezrin is of physiological significance. The probable rabbit homologue of human EBP50, the Na+/H+ exchanger regulatory factor, has been identified as a protein necessary for the cAMP-dependent protein kinase A regulation of the renal Na+/H+ exchanger (22, 23). A closely related protein, the NHE3 kinase A regulatory protein (E3KARP), was identified in a two-hybrid interaction screen using the cytoplasmic domain of the renal Na+/H+ exchanger NHE3 isoform as bait (24). Thus, a likely scenario places EBP50 as an adaptor protein between NHE3 and ezrin at least in the renal brush border. Very recently, EBP50 was identified in another two-hybrid screen, this time using the NH2-terminal domain of merlin as bait (12).
In this paper, we identify and characterize the regions in ezrin necessary for interaction with EBP50 and the regions in EBP50 necessary for an interaction with ezrin. Since the NH2-terminal domain of ezrin can bind both EBP50 and the ezrin C-ERMAD, we also examine the relationship between these binding sites. Our results show that the binding of EBP50 and the C-ERMAD to the ezrin NH2-terminal domain are mutually exclusive and hierarchical and that both binding sites are masked in the full-length molecule. The masking of the EBP50 binding site in dormant ezrin provides further biochemical evidence that ezrin has to be activated for its membrane-cytoskeletal linking function. These findings allow us to propose a model of molecular linkages that lead to the attachment of microfilaments to the plasma membrane.
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EXPERIMENTAL PROCEDURES |
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Production and Purification of Recombinant Proteins-- The design and production of the glutathione S-transferase (GST)-ezrin deletion series (18) and of the EBP50 and Ez-(1-296) constructs have been described (11). The full-length Ez-(1-585) and the Ez-(479-585) (C-ERMAD) constructs were created by polymerase chain reaction amplification of the respective cDNA sequences from clone F6 (4) using primers that generated EcoRI and HindIII sites at their ends. These products were then subcloned into the expression vector pQE16 (QIAGEN Inc., Chatsworth, CA). The series of GST-EBP50 proteins containing NH2- and COOH-terminal deletions was created by a combination of polymerase chain reaction amplification and subcloning of sequences from the human EBP50 cDNA (GenBankTM accession number AF015926). The polymerase chain reaction products that had been generated with unique restriction sites at their ends and the fragments to be subcloned were directionally ligated into the polylinkers of the appropriate pGEX series fusion vectors (Amersham Pharmacia Biotech). All recombinant sequences were determined to be free of polymerase chain reaction errors by nucleotide sequence analysis. Restriction enzymes and other reagents for molecular biology were purchased from Life Technologies, Inc.
The expression of the GST-ezrin series constructs (18) and of the Ez-(1-296) construct (11) has been described. GST-EBP50 deletion series constructs were transformed into the Escherichia coli strain DH5In Vitro Binding Assays-- Purified ezrin or Ez-(1-296) were covalently coupled to CNBr-activated Sepharose 4B (Sigma) at equal molar ratios (~4 mg/ml and ~2 mg/ml resin, respectively), as described (11). Glutathione-agarose beads with immobilized GST or GST fusion protein were prepared essentially according to the manufacturer's protocol (Amersham Pharmacia Biotech).
Soluble bacterial lysates were made by resuspending induced cells from 50 ml of culture in 1.2 ml of Tris-buffered saline (50 mM Tris, 150 mM NaCl, pH 7.4, at 4 °C) containing 50 µg/ml phenylmethylsulfonyl fluoride and 75 µg/ml benzamidine, lysing by sonication (Branson Ultrasonics Corp., Danbury, CT), and clarifying by centrifugation at 48,000 × g for 10 min. Binding assays were carried out by mixing 50 µl of a 25% slurry of coupled beads or glutathione fusion protein beads, with soluble induced bacterial cell lysate for 30 min at 4 °C. The beads were washed five times in 1 ml of Tris-buffered saline made up to 0.5 M NaCl, and bound proteins were extracted by boiling for 2 min in SDS sample buffer. For challenge reactions, the fifth wash after the first incubation with lysate was done in Tris-buffered saline made up to 150 mM NaCl, the beads were put through a second round of incubation and washing, and bound proteins were extracted. In the case where EBP50- or C-ERMAD-containing lysate was added in increasing amounts, reaction volumes were normalized with Tris-buffered saline.SDS-Polyacrylamide Gel Electrophoresis, Blot Overlays, and Immunoblots-- SDS-polyacrylamide gel electrophoresis was performed as described previously (25), and protein samples were analyzed on 10, 11, or 13.3% gels. In some cases, gels were stained with Coomassie Brilliant Blue R-250. For blots, proteins were transferred from gels to polyvinylidene membranes (Millipore Corp., Bedford, MA) using a semidry electroblotter (Integrated Separation Systems, Hyde Park, MA). All blots were developed using an enhanced chemiluminescence detection system (Amersham Pharmacia Biotech). In some cases, blots were stained with Coomassie Brilliant Blue R-250 after development to assess the efficiency of protein transfer.
Biotinylated Ez-(1-296) and EBP50 probes were prepared, and blot overlays were performed as described (17). The biotinyl probes were omitted in control experiments. Peroxidase-conjugated avidin (Sigma) was used to detect biotin-labeled proteins. Immunoblots were blocked with 10% nonfat dry milk, then probed with a 1:10000 dilution of GST antiserum (Amersham) in 1% milk, followed by 0.1 µg/ml peroxidase-conjugated goat anti-rabbit IgG in 1% milk. ![]() |
RESULTS |
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Mapping the Ezrin-EBP50 Interaction Sites-- The NH2-terminal domain of ezrin (Ez-(1-296)) binds to EBP50 with high affinity in solution and by blot overlay (11). To define the region in EBP50 that interacts with Ez-(1-296), a series of recombinant GST-EBP50 fusion proteins containing intact EBP50 or NH2- and COOH-terminal deletions, was generated and expressed in bacteria (Fig. 1). Analysis of lysates of induced bacteria show that the major induced polypeptides correspond to the GST fusion proteins (Fig. 1, upper and middle panels). Some of the GST-EBP50 fusion proteins exhibited an anomalously slow migration, like that seen for native EBP50 (11). Plots of RF versus log molecular weight indicated that the regions of EBP50 responsible for the majority of this retardation lie within residues 97-138 and 242-320. To determine the region in EBP50 necessary for association with Ez-(1-296), a blot overlay assay was employed in which biotinylated recombinant Ez-(1-296) was used as a probe on the GST-EBP50 fusion protein series (Fig. 1, bottom panel). The Ez-(1-296) probe bound only to those EBP50 constructs that contained an intact COOH terminus. A 61-residue COOH-terminal truncation was not recognized (Fig. 1, lane B), whereas all constructs that contained the COOH-terminal 30 residues (329-358) of EBP50 bound Ez-(1-296).
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The Binding Sites for EBP50 and the C-ERMAD Are Masked in the Native Ezrin-- The N-ERMAD (Ez-(1-296)) and C-ERMAD (Ez-(479-585)) of ezrin bind each other with high affinity in vitro. In native full-length ezrin, the C-ERMAD is masked and therefore unable to bind a free ectopic N-ERMAD (18). To explore whether or not the binding site for EBP50 in Ez-(1-296) is accessible in native ezrin, we compared the ability of full-length ezrin and Ez-(1-296) to bind recombinant EBP50. Additionally, since it has not been determined whether the N-ERMAD is accessible in full-length ezrin, we also compared the abilities of full-length ezrin and Ez-(1-296) to bind recombinant C-ERMAD.
Untagged, recombinant versions of full-length ezrin and Ez-(1-296) were expressed as soluble proteins in bacteria and purified to homogeneity (Fig. 4A). The purified proteins were then coupled covalently to beads to make affinity resins. Total soluble bacterial lysates expressing either a portion of the murine dihydrofolate reductase protein as a nonspecific control or untagged EBP50 or untagged C-ERMAD were prepared (Fig. 4B) and incubated with each set of beads. After extensive washing in high salt buffer, the bound proteins were eluted by boiling the beads in SDS sample buffer and analyzed by gel electrophoresis (Fig. 4C). Neither EBP50 nor the C-ERMAD bound to full-length ezrin (Fig. 4C, lanes 3 and 5, respectively), whereas both bound to Ez-(1-296) (Fig. 4C, lanes 4 and 6, respectively). No proteins from the control lysate bound to either set of beads (Fig. 4, lanes 1 and 2). Thus, the binding sites for EBP50 and an ectopic C-ERMAD are masked in native ezrin.
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EBP50 and the C-ERMAD Have Mutually Exclusive Binding Sites on Ez-(1-296)-- The region in ezrin required for binding EBP50 lies within residues 1-286 (Figs. 2 and 3), whereas the region necessary for binding the C-ERMAD lies in residues 1-296, with 1-286 being insufficient for this interaction (18). We therefore wished to determine whether Ez-(1-296) was able to bind EBP50 and the C-ERMAD simultaneously or if their binding was mutually exclusive.
Our strategy was to saturate immobilized Ez-(1-296) with EBP50 and then to examine whether EBP50 could be displaced by the subsequent addition of C-ERMAD. The quantity of EBP50-containing bacterial lysate needed to saturate all the Ez-(1-296) sites was determined by adding increasing amounts of lysate to replicate sets of beads. The beads were washed extensively, and bound EBP50 was eluted and analyzed by gel electrophoresis (Fig. 5A). Increasing amounts of lysate resulted in larger amounts of bound EBP50 (lanes 1-5) until a saturation point was reached where the addition of more lysate did not result in any further increase (lanes 6-7). This amount of EBP50-containing lysate was used to saturate replicate sets of Ez-(1-296) beads that were then challenged with increasing amounts of C-ERMAD-containing lysate (Fig. 5B). As the amount of lysate was increased, bound C-ERMAD increased and bound EBP50 decreased (lanes 1-5) until a point at which the addition of more C-ERMAD lysate did not result in any further increase in bound C-ERMAD (lanes 6-7). These results indicate that the C-ERMAD can displace the bulk of EBP50 from Ez-(1-296).
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DISCUSSION |
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In this study we have investigated the sites of interaction between EBP50 and ezrin. The results show that the COOH-terminal 30 residues of EBP50 are sufficient for an association with ezrin and that the EBP50 binding site in ezrin lies within the first 286 residues where it is masked in the native molecule. We have also shown that the binding of EBP50 to Ez-(1-296) can be inhibited by the C-ERMAD (Ez-(479-585)). These results have interesting implications for the modes of action of both EBP50 and ezrin.
Human EBP50 is 55% identical to human E3KARP, a 337-residue protein with two PDZ domains that interacts directly with the cytoplasmic domain of the Na+/H+ exchanger NHE3 isoform (24). The COOH-terminal 30 residues of EBP50 that bind ezrin are especially well conserved in E3KARP (Fig. 6), suggesting that E3KARP might also bind Ez-(1-296). This proposal is supported by preliminary experiments in which a GST-E3KARP fusion protein was found to bind Ez-(1-296) (or moesin residues 1-296) with high affinity.2 In addition, ezrin and band 4.1 have been reported to bind to hDlg (26, 27), the human homolog of the Drosophila discs large protein. Inspection of the region in hDlg believed to be responsible for this association revealed limited sequence identity to the COOH-terminal regions of EBP50 and E3KARP (Fig. 6). It is therefore possible that the nature of the interaction between ezrin and EBP50 is similar to that between ezrin or band 4.1 and hDlg.
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So far there is no evidence to indicate that the binding of EBP50 to Ez-(1-296) is regulated at the level of EBP50, since full-length and truncated forms of EBP50 containing the COOH-terminal 30 residues bind Ez-(1-296), and immobilized Ez-(1-296) binds to different phosphorylated forms of EBP50 present in tissue extracts (11). By contrast, the binding site for EBP50 is masked in full-length ezrin. When a series of bacterially expressed GST-ezrin deletion constructs were tested for their ability to bind an EBP50 probe in a blot overlay assay, all constructs containing ezrin residues 1-286 bound EBP50, with the remarkable exception of the full-length (1-585) construct. Removal of two COOH-terminal residues from ezrin restored the ability of EBP50 to bind it in the blot overlay assay (Fig. 2). The same phenomenon was seen when the binding of Ez-(1-583) and full-length ezrin to EBP50 were compared in solution (Fig. 4E). Since removal of these two residues destroys the ability of the C-ERMAD to bind the N-ERMAD (18), the most likely interpretation is that the C-ERMAD inhibits the binding of EBP50 to Ez-(1-296). We therefore suggest that in full-length ezrin, the C-ERMAD forms an intramolecular association with the N-ERMAD, thereby masking the potential EBP50 binding site in Ez-(1-296). Such a scenario would imply that EBP50 and the C-ERMAD cannot bind Ez-(1-296) simultaneously and that bound C-ERMAD cannot be displaced by soluble EBP50. These predictions are supported by our solution binding results (Figs. 4 and 5).
What is the relationship between the binding sites on Ez-(1-296) for EBP50 and the C-ERMAD (Ez-(479-585))? Several observations suggest that the two binding sites are not identical. First, the C-ERMAD requires ezrin residues 1-296 for full activity (18), whereas EBP50 binds to constructs containing only residues 1-286. The additional 10 residues needed for C-ERMAD binding are highly basic (pI = 10.98) and the C-ERMAD is more acidic (pI = 5.45) than the 30 residues in EBP50 sufficient for binding ezrin (pI = 10.56), suggesting that charge interactions in this region may be important for C-ERMAD binding. Second, immobilized Ez-(1-296) has sites that are accessible to EBP50 but not to the C-ERMAD. Third, there is no obvious sequence homology between the C-ERMAD and the COOH-terminal tail region of EBP50 that binds to Ez-(1-296). These results suggest that the binding sites are either distinct or overlap in such a way that binding of the C-ERMAD reduces the affinity of EBP50 for Ez-(1-296). If the sites are distinct, binding of the C-ERMAD must induce a conformational change in Ez-(1-296) that reduces its affinity for EBP50. Future structural analyses will be needed to distinguish unambiguously between these possibilities.
We have so far considered the interaction of Ez-(1-296) with EBP50 and the C-ERMAD. However, this same domain has also been reported to bind to both Rho-GDI (13) and the cytoplasmic tail of the transmembrane protein CD44 (10). Like EBP50, Rho-GDI can bind to a domain consisting of residues 1-286, and this binding can be abrogated by subsequent addition of a C-ERMAD (13). Since the C-ERMAD, EBP50, Rho-GDI, and the cytoplasmic tail of CD44 do not share any obvious sequence homology, it will be important to determine how many binding sites exist on Ez-(1-296) and, if mutually exclusive, what their binding hierarchy is.
How do these results relate to the current ideas of ezrin function? Previous studies have demonstrated that the C-ERMAD of ezrin, which contains the COOH-terminal F-actin binding site, is masked in the dormant full-length molecule (18). Moreover, the site in Ez-(1-296) for association with CD44 is partially masked in full-length ezrin (10) as is the site for association with Rho-GDI (13). In addition, we now show that the N-ERMAD is masked in the dormant full-length molecule. The finding that dormant ezrin does not bind EBP50, whereas EBP50/ezrin complexes can be isolated from purified placental microvilli (11), is strong evidence in support of a dormancy/activation model. Thus, the full-length molecule has the ability to assume a dormant conformation in which the COOH-terminal F-actin binding site, the self-association sites, and the association sites for EBP50, CD44, and Rho-GDI are all masked. Our current data suggest that this dormancy is due to an intramolecular N/C-ERMAD interaction, although other models are not formally excluded.
To function, the dormant ezrin monomer has to be activated to expose appropriate binding sites. At present the effectors of activation or the specific activation pathway have not been elucidated, although evidence exists to suggest that phosphatidylinositol 4,5-bisphosphate or tyrosine phosphorylation of ezrin might be involved (10, 20, 21, 28). One simple way to maintain the molecule in an activated state would be to inactivate the C-ERMAD by phosphorylation and thereby inhibit the proposed intramolecular association responsible for masking. The degree of phosphorylation of Thr-558 of moesin, which lies in the C-ERMAD, is enhanced during platelet activation, concomitant with an increase in cytoskeletally association moesin (29). Moreover, phosphorylation of the equivalent residue in ezrin, Thr-567, by Rho kinase abolishes C-ERMAD activity without affecting the COOH-terminal F-actin binding site (30). Thus, an ezrin molecule phosphorylated on Thr-567 would be predicted to bind F-actin through its COOH-terminal domain and EBP50 or CD44 through its NH2-terminal domain, thereby providing a molecular linkage between the membrane and cortical microfilaments. Since activation to expose binding sites is proposed to precede phosphorylation of Thr-567 (30), self-association through exposed N- and C-ERMADs can also be accommodated into this model. Oligomer formation could involve binding of an exposed C-ERMAD of one activated ezrin molecule to the N-ERMAD of a second activated molecule in a head-to-tail configuration (1, 21). If a C-ERMAD of an oligomer is phosphorylated, this would preclude the addition of another activated molecule at that end and allow the association with F-actin; the NH2-terminal end of the oligomer would have unmasked sites for association with EBP50, CD44, or Rho-GDI.
A recent report demonstrated that EBP50 binds to the NH2-terminal domain of merlin, a protein showing 61% sequence identity to ezrin over this region (12). We have also found that EBP50 will bind to bacterially expressed recombinant NH2-terminal domain (residues 1-313) of merlin.2 So far it is not known whether the affinity of EBP50 for merlin is as high as that for ezrin or whether the EBP50 binding site is masked in full-length merlin. Resolution of these points will determine how EBP50 is partitioned between ERM members and merlin and how this is altered by the stimulation of signal transduction pathways that activate ERM members. Thus, it appears that we are just beginning to glimpse the intricate and regulated nature of the associations in which the ezrin family of proteins can participate. Further studies will have to examine how ezrin selects among its many suitors, what the physiological role of each association is, and why a single protein participates in so many regulated associations.
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ACKNOWLEDGEMENTS |
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We are grateful to Dr. C. Yun for providing us with the GST-E3KARP fusion construct and to Dr. Mark Berryman for comments on the manuscript.
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FOOTNOTES |
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* This work was supported by National Institutes of Health Grant GM 36652.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Section of
Biochemistry, Molecular, and Cell Biology, Biotechnology Bldg., Cornell University, Ithaca, NY 14853. Tel.: 607-255-5713; Fax: 607-255-2428; E-mail: apb5{at}cornell.edu.
1 The abbreviations used are: ERM, ezrin-radixin-moesin; EBP50, ERM-binding phosphoprotein 50; N- and C-ERMAD, NH2-terminal and COOH-terminal ERM-association domain; GST, glutathione S-transferase; E3KARP, NHE3 kinase A regulatory protein; Rho-GDI, Rho-GDP dissociation inhibitor.
2 D. Reczek and A. Bretscher, unpublished data.
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REFERENCES |
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