Multiple Distinct Coiled-coils Are Involved in Dynamin Self-assembly*

Patricia M. OkamotoDagger , Brian Tripet§, Jennifer Litowski§, Robert S. Hodges§, and Richard B. ValleeDagger

From the Dagger  Department of Cell Biology, University of Massachusetts Medical School, Worcester, Massachusetts 01605 and the § Department of Biochemistry and the Medical Research Council Group in Protein Structure and Function, University of Alberta, Edmonton, Alberta T6G 2H7, Canada

    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Dynamin, a 100-kDa GTPase, has been implicated to be involved in synaptic vesicle recycling, receptor-mediated endocytosis, and other membrane sorting processes. Dynamin self-assembles into helical collars around the necks of coated pits and other membrane invaginations and mediates membrane scission. In vitro, dynamin has been reported to exist as dimers, tetramers, ring-shaped oligomers, and helical polymers. In this study we sought to define self-assembly regions in dynamin. Deletion of two closely spaced sequences near the dynamin-1 C terminus abolished self-association as assayed by co-immunoprecipitation and the yeast interaction trap, and reduced the sedimentation coefficient from 7.5 to 4.5 S. Circular dichroism spectroscopy and equilibrium ultracentrifugation of synthetic peptides revealed coiled-coil formation within the C-terminal assembly domain and at a third, centrally located site. Two of the peptides formed tetramers, supporting a role for each in the monomer-tetramer transition and providing novel insight into the organization of the tetramer. Partial deletions of the C-terminal assembly domain reversed the dominant inhibition of endocytosis by dynamin-1 GTPase mutants. Self-association was also observed between different dynamin isoforms. Taken altogether, our results reveal two distinct coiled-coil-containing assembly domains that can recognize other dynamin isoforms and mediate endocytic inhibition. In addition, our data strongly suggests a parallel model for dynamin subunit self-association.

    INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Dynamin is a high molecular mass GTPase (1, 2) that has been implicated in various aspects of endocytosis, including synaptic vesicle recycling, the endocytosis of assorted receptors, internalization of caveolae, and more recently budding from the trans-Golgi network (reviewed in Refs. 3 and 4). Dynamin belongs to a growing family of functionally diverse, large GTPases (4). In mammals, multiple isoforms of dynamin itself have been identified (4, 5), and functional dynamin homologs have been cloned from the lower eucaryotes Drosophila melanogaster (shibire; Refs. 6 and 7) and Caenorhabditis elegans (dyn-1; 8).

Dynamin self-assembly is critical to its function. It has been shown to form helical collars around the necks of coated pits (8) and is postulated to be involved in the subsequent budding of coated vesicles and other early endocytic intermediates. Structures corresponding to the helical collars can be formed in vitro from purified protein (9) as well as in combination with acidic substrata including microtubules (10), phospholipid tubules (11), and native synaptosomal membranes (12). Polymerization is concentration-dependent (13, 14) and inhibited in high ionic strength buffers (9). Self-assembly does not require guanine nucleotides (15, 16), although it is either stimulated or inhibited by them depending upon whether the protein is free or membrane-bound (15, 16). Once polymerized, dynamin can undergo a nucleotide-dependent conformational change that results in membrane fission in vitro (11). In the depolymerized state, dynamin has been reported to exist as either a dimer (16) or a tetramer (17) based on cross-linking studies. Analytical ultracentrifugation has favored tetramer as the predominant species (18).

The regions of dynamin that are important in self-association and in the interaction with lipids and other proteins have been a topic of considerable interest. Dynamin contains a highly conserved, N-terminal GTPase domain of ~300 aa1 and a centrally located pleckstrin homology (PH) domain that has been reported to bind to phosphatidyinositol 4,5-bisphosphate (19, 20) and G-protein beta gamma -subunits (21). Downstream of the PH domain are two predicted regions of coiled-coil alpha -helix, and at the C terminus is a 100-aa basic, proline-rich region to which Src homology 3 domains (22-24), acidic phospholipids (13), and microtubules (25) have been shown to bind. This domain has been implicated in targeting dynamin to coated pits through Src homology 3 domains (26).

Dynamin self-association stimulates its GTPase activity. Ligands that bind to the proline-rich domain stimulate both assembly and GTP hydrolysis, and removal of the domain inhibits both activities (13, 22, 25). More recently, proteolytic dynamin fragments missing the proline-rich domain were shown by electron microscopy to be capable of self-assembly when in the presence of GDP and metallofluorides at physiological salt conditions (27) or on lipid bilayer tubes (11).

The role of the putative coiled-coil sequences in dynamin self-association is uncertain. Coiled-coil probability is only ~60% (see "Results"), and whether this region actually forms coiled-coil structure, amphipathic alpha -helix, or neither is uncertain. This region is conserved among the dynamin isoforms and dynamin-related proteins (4), and computer-based analysis (Newcoils; Ref. 28) predicts comparable secondary structure in all of these proteins. The dynamin-related Mx proteins exhibit clear heptad repeats within this region consistent with a leucine zipper structure that, when fused to a reporter gene, was capable of self-association (29).

A potential role for the putative coiled-coil region of dynamin emerged from our previous analysis of the inhibitory endocytic phenotype in mammalian cells transiently transfected with a dominant negative, C-terminal deletion mutant (30, 31). Inhibition was unaffected by removal of the proline-rich domain but was reversed by further deletion into the putative coiled-coil region, suggesting that this part of the molecule might mediate the interaction of mutant dynamin with the endogenous wild-type protein (31). To gain further insight into the mechanism underlying the inhibitory phenotype and to understand the mechanism of dynamin self-association, we have used a series of deletion mutants to define sites of dynamin self-association and identify two distinct regions. Analysis of peptides reveals that at least three sequences in dynamin-1 are capable of self-association. These results suggest a critical role for the coiled-coil region in dynamin self-assembly.

    EXPERIMENTAL PROCEDURES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

cDNA Constructs-- The dynamin-1ab isoform (1) was used for most experiments. C-terminal and internal deletion mutants were made via polymerase chain reaction and subcloned into the mammalian expression vector, pSVL (Amersham Pharmacia Biotech). Polymerase chain reaction was also used to fuse the HA (32) or Myc epitope (33) to the N terminus, and all constructs were sequenced to ascertain that the mutations and epitope tags were correct. The dynamin-2bb isoform (31) was also Myc-tagged at the N-terminal end using polymerase chain reaction.

Co-Immunoprecipitation Assay for Dynamin Self-association-- For the co-immunoprecipitation assays, COS-7 cells were transiently transfected with both HA- and Myc-tagged dynamin-1 constructs using the LipofectAMINE reagent (Life Technologies, Inc.) as directed by the manufacturer. Cytosolic extracts of the co-expressed proteins were prepared by lysing the transfected cells in RIPA buffer (50 mM Tris, pH 7.4, 150 mM NaCl, 1% Nonidet P-40, 1 mM phenylmethylsulfonyl fluoride, 1 µg/ml aprotinin, 1 µg/ml leupeptin) and clearing the lysates at 30,000 × g and 4 °C for 20 min to remove any cellular debris. After preclearing the supernatants with protein A beads (Amersham Pharmacia Biotech) for several hours, fresh protein A beads were added along with either anti-HA monoclonal antibody (Babco, Berkeley, CA) or anti-Myc polyclonal antibody (a gift of Dr. Melissa Gee, University of Mass. Medical School, Worcester, MA). Co-immunoprecipitation assays were carried out overnight at 4 °C with end-over-end rotation, after which the beads were washed several times in NET gel buffer (50 mM Tris, pH 7.4, 150 mM NaCl, 1 mM EDTA, 0.25% gelatin, 0.1% Nonidet P-40) and then resuspended in an equal volume of SDS sample buffer for SDS-polyacrylamide gel electrophoresis. Western analysis was done using either the HA monoclonal antibody (Babco) or the Myc monoclonal antibody (9E10, ATCC), and chemiluminescence was used to detect any protein interactions (Kirkgaard and Perry Laboratories).

Yeast Interaction Trap-- The LexA-based interaction trap (34) was kindly provided by Dr. Erica Golemis (Fox Chase Cancer Center, Philadephia, PA) and used to assay for dynamin-dynamin interactions in yeast. Wild-type dynamin-1 was subcloned into the JG202 bait expression vector, which contains a nuclear localization signal. Wild-type and deletion mutants of dynamin were constructed in the JG4-5 prey vector. We tested the suitability of the wild-type dynamin-1 in JG202 as bait and found that it did not activate transcription alone. The lithium acetate method was used to make yeast competent cells and for transformations (35). Dynamin-dynamin interactions were scored positive if transcription of the lacZ and LEU2 reporter genes were activated.

Sucrose Density Gradient Centrifugation-- Sucrose density gradients (5-20%) were prepared in 20 mM Tris, pH 7.4, 50 mM KCl buffer. Cytosolic extracts of COS cells transfected with Myc-tagged dynamin constructs were prepared as described above. For each gradient, 500 µg of the extract and 10 µg of each molecular mass marker (Sigma) were loaded. Centrifugation was at 26,500 rpm and 4 °C for 17 h. Fractions were collected at 20-s intervals and analyzed by SDS-polyacrylamide gel electrophoresis. Detection of dynamin was by chemiluminescence using a Myc monoclonal antibody. The positions of the molecular mass markers in the gradients were detected by Coomassie stain. Densitometric measurements were made on a Bio-Rad model GS-700 Imaging Densitometer scanner interfaced to the Bio-Rad Multi-analyst computer program (version 1.1). Protein concentrations were determined by the Bradford assay (Bio-Rad), and the S values for the markers are as follows: bovine serum albumin, 4.5 S; alcohol dehydrogenase, 7.5 S; beta -amylase, 9 S.

Endocytosis Assays-- Transferrin uptake was measured in COS cells as described previously (30) with the following modifications. After transient transfection of the cells with Myc-tagged dynamin constructs, the cells were grown in serum-free medium for 24 h. Transferrin endocytosis was then stimulated by adding 20 µg/ml of fluorescein isothiocyanate-labeled transferrin (Molecular Probes) for 10 min at 37 °C, after which uptake was stopped by placing the cells on ice and washing several times with ice-cold phosphate-buffered saline. Cells were then fixed with 4% paraformaldehyde for 15 min at room temperature and subsequently extracted with either ice-cold methanol for 5 min or 0.5% Triton X-100 for 2 min. Cell staining was done as described previously (30), and immunofluorescent imaging was with a Zeiss Axiophot microscope.

Peptide Synthesis and Purification-- Synthetic peptides were prepared by solid phase synthesis methodology using a 4-benzylhydrylamine hydrochloride resin with conventional N-t-butyloxycarbonyl chemistry on an Applied Biosystems model 430A peptide synthesizer as described by Sereda et al. (36). Peptides were cleaved from the resin by reaction with hydrogen fluoride (20 ml/g resin) containing 10% anisole and 2% 1,2-ethanedithiol for 1 h at -5 °C, washed with cold ether several times, extracted from the resin with glacial acetic acid, and then lyophilized. Purification of each peptide was performed by reversed-phase chromatography on a Syn-Chropak semi-preparative C-8 column (inner diameter, 250 × 10 mm; 6.5-µm particle size; 300-Å pore size; SynChrom, Lafayette, IN) with a linear AB gradient (ranging from 0.2 to 1.0% B/min) at a flow rate of 2 ml/min, where solvent A is aqueous 0.05% trifluoroacetic acid and solvent B is 0.05% trifluoroacetic acid in acetonitrile. Homogeneity of the purified peptides was verified by analytical reversed-phase chromatography, amino acid analysis, and electrospray quadrapole mass spectrometry.

Circular Dichroism Spectroscopy-- CD spectra were recorded on a Jasco J-720 spectropolarimeter (Jasco, Inc.) interfaced to an Epson Equity 386/25 computer running the Jasco DP-500/PS2 system software (version 1.33a). The temperature-controlled cuvette holder was maintained at 20 °C with a Lauda model RMS circulating water bath. The instrument was calibrated with an aqueous solution of recrystallized d-10-(+)-camphorsulfonic acid at 290.5 nm. Results are expressed as the mean residue molar ellipticity [theta ] (degrees·cm2·dmol-1) calculated from the following equation.
[&thgr;]=(&thgr;<SUB><UP>obs</UP></SUB>−M)/(10×l×c) (Eq. 1)
where theta obs is the observed ellipticity expressed in millidegrees, M is the mean residue molecular mass (molecular mass of the peptide divided by the number of amino acids), l is the optical path length in centimeters, and c is the final peptide concentration in mg/ml. The CD wave scans were measured from 190 to 255 nm in benign buffer (0.1 M KCl, 0.05 M potassium phosphate, 2 mM dithiothreitol, pH 7) at two peptide concentrations, 1 and 0.1 mM, unless otherwise noted in the text. For samples containing TFE, the above buffer was diluted 1:1 (v/v) with TFE.

Sedimentation Equilibrium Analytical Ultracentrifugation-- Sedimentation equilibrium ultracentrifugation was performed on a Beckman model XLI Analytical Ultracentrifuge and interference optics as described in the instrument manual (Beckman Instruments). Samples were dialyzed against and run in a 50 mM potassium phosphate, 100 mM KCl, 2 mM dithiothreitol, pH 7 buffer. Six-sector charcoal-filled epon sample cells were used, allowing three concentrations of sample to be run simultaneously. Runs were performed at two or three speeds between 20,000 and 32,000 rpm and were continued until there was no significant difference in scans taken 2 h apart. The data were evaluated using a nonlinear least squares curve-fitting algorithm (37) contained in the NonLin analysis program. The program Sednterp (Sedimentation Interpretation Program, version 1.01) was employed to calculate the partial specific volume of the protein from the amino acid composition as well as the solvent density and viscosity using known values from physical tables.

    RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Assays for Dynamin Self-association-- As a first step in defining a self-association domain in dynamin-1, we tested for interactions between epitope-tagged dynamin-1 constructs co-expressed in COS cells. Full-length Myc- and HA-tagged wild-type dynamin-1 (C851; Fig. 1, A and B; see also Fig. 7) were observed to co-immunoprecipitate using antibody recognizing either epitope. Co-immunoprecipitation was still observed with C-terminal deletions that were lacking all or part of the proline-rich region (C750; Fig. 1, A and B; see also Fig. 7) as well as with mutants missing either the GTPase (N272; see Fig. 7) or the PH domain (Delta PH; Fig. 1C; see also Fig. 7). In contrast, co-immunoprecipitation was abolished by a C-terminal deletion which removed the second of the two potential coiled-coil forming segments (C695; Fig. 1, A and B; see also Fig. 7). Co-immunoprecipitation was also eliminated by internal deletions that removed the first of the two regions or both together (Delta CC1 or Delta CC12; Fig. 1C; see also Fig. 7). These data suggested that the sequence between aa 654 and aa 741 containing the two regions may represent an important self-assembly domain.


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Fig. 1.   Co-immunoprecipitation of HA- and Myc-tagged dynamin-1 constructs. Co-immunoprecipitations (i.p.) of HA- and Myc-tagged dynamin-1 constructs were performed using a Myc polyclonal antibody. Interactions were detected with either the Myc or HA monoclonal antibodies. The blots in panel A are probed with the HA mAb (lot L), those in panel B are probed with the Myc mAb, and those in panel C are probed with the HA mAb (lot N). The cross-reacting band observed in panel C was lot-specific. In panels A and B, co-immunoprecipitation was assayed between HA- and Myc-tagged C-terminal deletion mutants of similar lengths, whereas in panel C, Myc-tagged dynamin-1 internal deletion mutants were co-immunoprecipitated with full-length HA-tagged dynamin-1. The boundaries for the internal deletion mutants shown in panel C are as follows: Delta PH, aa 514-629; Delta CC1, aa 654-681; Delta CC12, aa 654-741. C851, full-length dynamin-1; B, beads alone, control.

As an alternative approach to defining interaction sites, we also used a yeast two-hybrid system. Interactions were assayed between a wild-type dynamin-1 bait and a panel of dynamin-1 deletion mutant prey constructs. In agreement with the co-immunoprecipitation results, dynamin-1 preys that were missing part of the proline-rich region still interacted with the wild-type dynamin-1 bait (C761; Fig. 2; see also Fig. 7), although deletion of the entire proline-rich region resulted in little, if any, interaction (C750; Fig. 2; see also Fig. 7). We also detected a reduction in interaction intensity with a C-terminal deletion mutant (C733; Fig. 2; see also Fig. 7) that had previously been shown to reverse the dominant negative endocytic effect of K44E (30). As had been observed in the co-immunoprecipitation experiments, interactions persisted in prey devoid of either the GTP-binding domain (N272; Fig. 2; see also Fig. 7) or the PH domain (Delta PH; Fig. 2; see also Fig. 7). C-terminal deletions missing some or all of the potential coiled- coil forming sequences resulted in no interaction with the full-length bait (C695, C648, and C514; Fig. 2; see also Fig. 7) as did partial or complete removal of the coiled-coil region between aa 654-741 (Delta CC1, Delta CC2, and Delta CC12; Fig. 2; see also Fig. 7), consistent with our co-immunoprecipitation data.


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Fig. 2.   Assay for dynamin-dynamin interaction using the yeast interaction trap. Dynamin-dynamin interactions were assayed in the yeast strain EGY48 using a full-length dynamin-1 bait and dynamin-1 deletion mutant preys. Interactions were assayed on galactose plates lacking uracil, histidine, and tryptophan in the presence of 5-bromo-4-chloro-3-indolyl beta -D-galactopyranoside. Blue colonies are positive; non-blue colonies are negative. The nomenclature of the various mutants are the same as in Fig. 1. JG4-5 refers to the prey vector alone.

These data were consistent with our hypothesis that dominant inhibitory dynamin polypeptides act through interaction with endogenous wild-type dynamin protein (30). To test this possibility directly, we assayed for transferrin uptake in cells overexpressing dominant negative dynamin-1 K44E mutants that also had deletions in the self-assembly region. Fig. 3 shows that removal of either of the two self-association sequences identified in our co-immunoprecipitation and yeast interaction trap assays resulted in reversal of the dominant negative endocytic phenotype, i.e. the resumption of transferrin uptake. Because dynamin-1-K44E exhibits its inhibitory effects in cells containing primarily the dynamin-2 and dynamin-3 isoforms (30), we also tested for an interaction between isoforms. Interaction between dynamin-1 and dynamin-2 could be readily detected both by the yeast two-hybrid assay (Fig. 4A) and by co-immunoprecipitation (Fig. 4B).


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Fig. 3.   Reversal of endocytic inhibition by deletion of assembly sequences. Fluorescein isothiocyanate-transferrin internalization was measured in COS-7 cells transiently transfected with wild-type dynamin-1 (WT), a dominant inhibitory mutant form of dynamin-1 (K44E), or internal deletions of either of the latter construct (K44E/Delta CC1 or K44E/Delta CC2). All constructs were Myc-tagged, and their expression was detected by the Myc monoclonal antibody 9E10. Transferrin internalization is inhibited in the cell overexpressing the K44E mutant construct but is restored in cells expressing the doubly mutant constructs.


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Fig. 4.   Heterotypic interaction between the dynamin-1 and dynamin-2 isoforms. A, dynamin-2 (Dyn-2) bait was tested for an interaction with the dynamin-1 (Dyn-1) prey or with the JG4-5 vector as a control. Selection was on galactose lacking uracil, histidine, and tryptophan in the presence of 5-bromo-4-chloro-3-indolyl beta -D-galactopyranoside medium. B, co-immunoprecipitation of dynamin isoforms. Myc-dynamin-2 and HA-dynamin-1 were co-expressed in COS-7 cells and immunoprecipitated using the Myc polyclonal antibody. C, beads alone, control. D, anti-Myc immunoprecipitants blotted with Myc (left) polyclonal or HA (right) monoclonal antibody. The arrow points to the dynamin isoform in each blot. IgG, cross-reacting antibody heavy chain.

To learn more about the identity of the dynamin self-association products, lysates of COS-7 cells expressing either epitope-tagged wild-type or mutant dynamin-1 were analyzed by sucrose density gradient centrifugation. We established that the COS-expressed Myc-tagged dynamin-1 isoform behaved similarly to rat brain dynamin-1 in the sucrose density gradients (data not shown). Both ran as a 7.5 S peak, indicating that they were not in a highly assembled state under these conditions. The S value was unaffected by the removal of either the proline-rich (Fig. 5A; see also Fig. 7) or PH domains (Fig. 5B; see also Fig. 7). However, deletions involving the self-assembly region identified by our co-immunoprecipitation and yeast interaction trap experiments resulted in a shift of the 7.5 S peak to 4.5 S (C695; Fig. 5A; see also Fig. 7; and Delta CC12; Fig. 5B; see also Fig. 7), consistent with dissociation to a smaller species. No such shift was produced by deletion to aa 733 (C733; Figs. 6 and 7), which reverses the dominant inhibitory endocytic effect (31), despite removal of several amino acids from the C terminus of the self-assembly domain. However, partial dissociation was observed in a different gradient buffer (20 mM Hepes, pH 7, 50 mM KCl; Figs. 6 and 7). These results indicated a decrease in the affinity between polypeptides, although the ability to self-associate was not abolished completely.


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Fig. 5.   Sucrose density gradient centrifugation of various dynamin-1 C-terminal deletion mutants. COS-7-expressed Myc tagged dynamin-1 constructs were analyzed in 5-20% sucrose density gradients and immunoblotted using anti-Myc antibody. The blots were quantified by densitometry. The densitometric scans were normalized for expressed protein concentration for each construct. S values for markers used are shown at the top. A, data for full-length dynamin-1 (C851) and C-terminal deletions C750 and C695. B, data for full-length dynamin-1 (C851) and the internal deletions Delta PH and Delta CC12.


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Fig. 6.   Buffer-dependent dissociation of C733. The C-terminal dynamin-1 truncation construct C733 was analyzed in 5-20% sucrose density gradients containing either the standard gradient buffer (20 mM Tris, pH 7.4, 50 mM KCl) (A) or 20 mM Hepes, pH 7, 50 mM KCl (B). Other conditions are as described in the legend to Fig. 5.


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Fig. 7.   Summary of the mapping results. Schematic representation summarizing the cDNA constructs used to map the C-terminal self-assembly region by co-immunoprecipitation (Co-IP), yeast two-hybrid (2-Hybrid), and sucrose density gradients (S-value). ++, very good interaction; +, good interaction; +/-, detectable interaction; -, no interaction; Pro-rich, proline-rich domain.

Peptide Analysis-- The domain implicated in dynamin-1 self-assembly contains two short, closely spaced sequences (aa 654-681 and aa 712-740) predicted by the Newcoils program (28) to have a propensity for coiled-coil formation based on analysis of a data base of known coiled-coil sequences (Fig. 8A). However, the probability is only ~60%, with no more than four heptad repeats predicted for each region. Newcoils also predicts at even lower probability three short sequences downstream of the GTPase domain between aa 295-470 (Fig. 8A). Paircoils, which is based on pairwise residue correlations (38) yielded a very different set of predictions, including a short sequence in near the center of the dynamin-1 polypeptide (Fig. 8B). Because of the disparity in the two predictive approaches, we also examined dynamin-1 using a recently developed nonstatistically based algorithm termed Stablecoils, which is based on the direct analysis of coiled-coil formation by synthetic peptides of systematically varied composition (39). The aa 651-675 region was judged to be the most hydrophobic with the highest propensity for amphipathic helix formation (Fig. 8C). A lower, but significant, propensity for coiled-coil formation was observed for aa 715-738, and additional sequences were identified in the central portion of the polypeptide that differed from those identified by Newcoils and Paircoils (Fig. 8).


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Fig. 8.   Secondary structure analysis. Newcoils (A), Paircoils (B), and Stablecoils (C) plots of dynamin-1 are shown, along with sequences selected for the design of synthetic peptides (bottom).

To determine which of these short sequences in fact had properties consistent with coiled-coil formation, we analyzed synthetic peptides corresponding to five distinct regions by circular dichroism and equilibrium ultracentrifugation (Table I). The CD spectrum of the D1 peptide, which was derived near the GTPase domain of the dynamin-1 polypeptide, was predominantly random coil. We note, however, that in 50% TFE, a helix-inducing hydrophobic solvent, it could be forced into an alpha -helical conformation, indicating that this region of dynamin has the intrinsic ability to adopt a helical secondary structure (data not shown). Similarly, the centrally derived D5 peptide exhibited a mixture of random coil and beta -sheet, but not alpha -helical, structure in benign solution (Fig. 9A). In contrast, peptides D2, D3, and D4 exhibited alpha -helical CD spectra, with the characteristic minima at 208 and 222 nm (Fig. 9B). An increase in alpha -helicity (10-20%) was observed for the D2 and D4 peptides at higher concentrations, whereas limited solubility of D3 precluded comparable analysis. CD spectra for a mixture of D2 and D4 were additive (data not shown). Curiously, D3/D4 or D2/D3 mixtures were less than additive (data not shown). This may be due to nonspecific interactions by D3, which also caused a similar, but smaller, decrease in the mean residue molar ellipticity at 222 nm when mixed with a known coiled-coil forming peptide from an unrelated protein, MMKif (Ref. 39 and data not shown). Peptides D2, D3, and D4 all exhibited low stability and were completely unfolded at low concentrations of guanidine HCl (0.75 M; Fig. 10). Table II summarizes the CD data.

                              
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Table I
Amino acid sequences of the synthetic peptides used in this study


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Fig. 9.   CD spectra of peptides D1-D5. Dynamin-1 peptides D1 and D5 (100 µM), which correspond to aa 295-318 and aa 372-404, respectively (A), and peptides D2, D3, and D4, which correspond to aa 323-352, aa 652-681, and aa 712-740, respectively (B), were analyzed at 20 °C in benign buffer (0.1 M KCl, 0.05 M potassium phosphate, 2 mM dithiothreitol, pH 7). Petides D2, D3, and D4 showed characteristic alpha -helical spectra.


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Fig. 10.   Denaturation of dynamin-1 peptides D2, D3, and D4. CD spectra of the three helical dynamin peptides D2, D3, and D4 in benign buffer at increasing molar concentrations of guanidine HCl. Peptide concentrations were 0.32, 0.07, and 0.47 mg/ml for D2, D3, and D4, respectively. The fraction folded of each peptide was calculated as f = ([theta ]obs - [theta ]u)/([theta ]f - [theta ]u) where f is the fraction folded, [theta ]obs is molar ellipticity observed for a given [guanidine HCl], [theta ]u is the molar ellipticity of the unfolded state, and [theta ]f is the molar ellipticity of the folded state.

                              
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Table II
Ellipticities and stabilities of the synthetic peptides

Equilibrium ultracentrifugation of peptides D2, D3, and D4 revealed that each is capable of oligomerization. The sedimentation data for D2 and D4 each fit to a homogenous species with mass average molecular masses of 14,051 and 15,210 Da, respectively, in both cases consistent with the formation of a tetramer (Fig. 11, A and B). D3 was observed to have a mass average molecular mass of 23,873 Da, which approaches a hexameric species (Fig. 11C). This suggests that D3 may not have a strictly defined oligomeric state but does have the ability to form helical bundles.


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Fig. 11.   Equilibrium ultracentrifugation of helical peptides. A, peptide D2. B, peptide D4. C, peptide D3. Peptide concentration gradients are shown and fit to a tetramer (A and B), and hexamer for C. Residuals (top) show deviation of measured points from fit line. Insets, peptide concentration gradients compared with theoretical lines for monomer (M), dimer (D), tetramer (T), or hexamer (H). The data for peptides D2 and D4 (A and B) fit to a tetrameric species, whereas those for peptide D3 fit to a hexamer (C). Sedimentation runs were at 25,000, 22,000, and 25,000 rpm, for D2, D3, and D4, respectively. r2/2, radial distance; ln(y), natural log of fringe displacement (concentration).


    DISCUSSION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Our results implicate two portions of dynamin in self-association, a complex region located between the PH and proline-rich domains and a region near the center of the polypeptide (Fig. 12A). We will refer to these regions as the C-terminal and central self-assembly domain, respectively. Our peptide analysis further identified coiled-coil forming sequences within both regions (Fig. 12A) and implicates coiled-coils as a primary mode of dynamin-dynamin interaction. Our results confirm our hypothesis that the C-terminal region mediates the interaction between dominant inhibitory dynamin mutants and endogenous wild-type protein. Furthermore, the identification of two distinct coiled-coil domains has important implications for dynamin structural organization, as discussed below.


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Fig. 12.   Models for the structural organization of dynamin tetramers. A, summary of peptide analysis. Dark bars, location of peptides that were alpha -helical by CD analysis; dotted bars, location of peptides that were random coil or a mixture of random coil and beta -sheet by CD; Assembly, self-assembly regions identified in this paper; R, shortest C-terminal deletion (aa 733) at which receptor-mediated endocytosis is observed in a dominant negative dynamin-1 mutant (see Ref. 31). B, dynamin-1 polypeptides are shown either in a parallel (model I) or anti-parallel (model II) orientation with coiled-coil sequences corresponding to peptides D2, D3, and D4 linking the individual polypeptides together.

Nature of Self-assembly Species-- A significant issue in this study is the stage in self-assembly in which these regions participate. Dynamin has been reported to exist in the unassembled state primarily as a tetramer (14, 16), although whether this species represents a stable, minimal assembly unit is unclear. Dynamin and the Mx proteins also assemble to partial rings, complete rings, and helical stacks of rings. Our analysis has dealt primarily, if not exclusively, with dynamin in the disassembled state. Our immunoprecipitation studies were performed at a sufficiently high ionic strength range to prevent assembly (14). The sucrose gradient analysis, although performed at lower ionic strength, revealed directly that the protein was in the disassembled state. The S value of 7.5 is consistent with a tetramer, albeit a highly assymetric structure. This species is clearly oligomeric in view of the sharp decrease in S value caused by small changes in C-terminal sequence. The state of self-association of dynamin-1 expressed in yeast is uncertain. The N-terminal fusion sequences could inhibit assembly, although N-terminal GFP-dynamin appears to function normally in cells (5).2 Because our mapping studies are so closely consistent with the results of our co-immunoprecipitation and centrifugation analysis, it is likely that the two-hybrid analysis primarily reflects monomer-dimer or monomer-tetramer formation, with one intriguing exception.

Previous studies of dynamin pointed to a role for the proline-rich domain in dynamin self-assembly (9, 14, 16). However, in these cases effects on polymer formation were assayed. Our data indicate that the proline-rich region is not required for self-association to the dimer or tetramer level; hence, it must be required for higher order assembly steps. We did observe diminution in the intensity of the yeast two-hybrid reaction using the C750 construct in the prey vector (Fig. 2), although the extent of co-immunoprecipitation was not affected by a comparable deletion, nor was the mutant protein observed to dissociate to the 4.5 S species by sucrose density gradient centrifugation. How the yeast result is to be interpreted is unclear. It may indicate greater sensitivity in detecting changes in affinity between dynamin subunits, or it may indicate that some extent of co-polymerization of bait and prey dynamin does actually occur in this system. We do note that although we tested for interactions between identical truncation mutant constructs in our other assays, full-length bait was used in the two-hybrid analysis. Thus, it is also possible that interaction between wild-type and the C750 mutant dynamin could be sterically affected by the proline-rich region.

The GTPase and PH domains were not required for dynamin self-association in our assays. The former result contrasts with those for the antiviral Mx proteins. Among the dynamin-related family members, the structure of these proteins has been the most extensively characterized. Three self-assembly regions have been mapped within the Mx1 protein. The monomer-to-polymer transition was assayed by gel filtration chromatography of full-length and truncation mutant Mx constructs. This analysis identified one self-assembly site within the GTPase domain (40) and a second near the C terminus (29). No role was detected for a putative leucine zipper domain further downstream at the extreme C terminus. In contrast, the latter region was implicated in dimerization in a separate study in which it was fused to a reporter enzyme. The basis for the difference in these results is unclear. The latter results, however, seem to be more nearly consistent with our findings for dynamin. Although we find no obvious sequence homology between the leucine zipper region of Mx and the C-terminal assembly domain of dynamin, their secondary structures seem to be related. Thus, it is likely that C-terminal coiled-coils may play a common role throughout the greater dynamin protein family, a conclusion supported by secondary structure predictions for other family members (41).

Role of Coiled-coils-- Secondary structure predictions for dynamin-1 by the Newcoils, Stablecoils, or Paircoils algorithms suggested several possible coiled-coil regions in dynamin-1, although the predictions differed substantially. We tested the ability of five of these regions to form interacting alpha -helical structure using synthetic peptides. Intriguingly, the predictive success of each algorithm was variable. It is not yet clear whether this outcome reflects the choice of peptide boundaries or features of the predictive schemes. Three of the five peptides exhibited clear evidence for alpha -helix formation by CD spectroscopy: D3 and D4 within the C-terminal self-assembly domain, identified in our analysis of recombinant dynamin polypeptides, and D2, derived from the center of the polypeptide. D3 was predicted to have a 60% probability of coiled-coil formation by Newcoils, only 11% probability by Paircoils, and the strongest propensity for coiled-coil formation using Stablecoils. D4 also exhibited 60% probability using Newcoils and approximately half the propensity of D3 using Stablecoils. Results were most surprising for the other peptides. D2 showed insignificant probability using Newcoils, only slightly positive probability using Stablecoils, and 11% using Paircoils. We considered D1 worth examining because, despite moderate predictive scores from Newcoils and Stablecoils, the homologous region within dynamin-2 exhibited 95% probability using Newcoils. Nonetheless, the D1 peptide was observed as a random coil by CD. It is possible that the coiled-coil forming sequence within the complete dynamin-1 polypeptide is more extensive, encompassing the D1 region and other regions as well.

In the case of the C-terminal assembly domain our data support the existence of two short stretches of alpha -helix (D3 and D4) separated by a 31-aa intervening sequence of undetermined structure (pI = ~5.3). Whether this region also participates in coil formation is uncertain; however, the D3 coil cannot be much longer than predicted because proline residues flank the sequence on either side. Although the sequence of this C-terminal assembly domain is conserved among the dynamin isoforms (79%), only the D3 region is consistently predicted by the Newcoils program to form a potential coiled-coil, albeit with varying probability (42-60% between rat dynamin isoforms). It is of interest that the D4 region has very low coiled-coil probability in dynamin-2. Inspection of the latter sequence suggests that a single amino acid gap accounts for this difference. That dynamin-2 co-immunoprecipitated with dynamin-1 is significant; this result implies that isoforms are interchangeable in the cell. It helps to explain the dominant inhibition of endocytosis by heterologous isoforms. In addition, it raises questions about models that implicate dynamin isoforms in distinct cellular functions (5). Conceivably, targeting signals exist that override the tendency toward miscibility and segregate isoforms to different membranous compartments. However, dynamins appear to be predominantly cytoplasmic (26), where our results suggest they would be free to intermix. Finally, deletion of either of these regions in the dynamin-1-K44E mutant reversed the dominant negative endocytic effect and resulted in transferrin uptake, indicating that these regions are indeed functionally important.

CD spectra of mixtures revealed no obvious evidence for heterodimerization. However, despite their relatively short lengths, peptides D2, D3, and D4 all clearly self-associated. D2 and D4 were observed to be tetrameric, with no evidence for higher order aggregates. That self-association involved coiled- coil formation is supported by the increase in alpha -helical content with concentration for at least two of the three peptides. D3 associated to a somewhat nonhomogenous mixture that was predominantly hexameric, with evidence of dissociation to smaller species in the lower concentration range. Because this peptide exhibited other evidence of nonspecific binding, caution must be exercised in interpreting its self-association behavior. It is possible that in the context of the entire protein, the D3 region is constrained to a four-stranded coiled-coil like the other regions. The self-association behaviors of D2 and D4 are particularly interesting in light of evidence that dynamin may exist in the depolymerized state as a tetramer. Our results not only add strong support to the latter claim but also suggest that the coiled-coil regions are sufficient for dynamin tetramerization.

Structural and Physiological Role of Assembly Domains-- How the dynamin self-assembly regions are distributed within the folded tetramer is unknown. Two general models may be envisioned depending on whether the alpha -helices are arrayed in parallel or anti-parallel. In the first case, we imagine that each of the three coiled segments, corresponding to D2, D3, and D4, participates in the formation of a tetrameric backbone with uniformly oriented polypeptides. Such an arrangement is clearly feasible (Fig. 12B, model I) and has a number of interesting structural consequences. For one, the tetramer would have structural polarity, a property required for the formation of a polymer with distinct membranous and cytoplasmic surfaces as may be expected for dynamin (10, 11). In addition, it may be argued based on symmetry considerations that the coiled-coil regions must be co-linear. Thus, we would predict that the dynamin tetramer is organized about a central coiled-coil shaft. It is also possible that the central and C-terminal self-assembly regions function at different levels of dynamin self-association, although the fact that both D2 and D4 form tetramers makes such models seem less likely. Our existing evidence indicates that the C-terminal region is important in the monomer-dimer or monomer-tetramer transition; conceivably, the central assembly domain might be involved in polymer formation. Although this is an attractive possibility, it would lead to network formation among dynamin polypeptides, inconsistent with the known features of the dynamin self-assembly pathway. Similar problems arise for models in which the peptides are proposed to interact in anti-parallel (Fig. 12B, model II). In particular, it is difficult to see how interaction of both assembly domains could occur between polypeptides in an antiparallel manner. Thus, we strongly favor the parallel model.

It is of interest that the C-terminal self-assembly domain appears to lie within the boundaries of a previously identified 13-kDa proteolytic fragment of dynamin-1 implicated in GTPase regulation. This fragment, termed the GED (GTPase effector domain) was found to bind to the GTPase domain and stimulate its activity (18). Whether the coiled-coil sequences we have identified within this fragment or additional sequences within this region are involved in GTPase effector activity is uncertain, and how self-association influences this interaction remain to be seen. However, it now seems clear that the coiled-coil segments of dynamin represent a new, functionally important element. Further analysis of these regions should be of considerable value in understanding how assembly of this remarkable protein is controlled.

    ACKNOWLEDGEMENTS

We thank Dr. Chantal Gamby for the schematic diagram of dynamin organization and for helpful comments and discussion on the manuscript. We also thank other members of the Vallee lab, Dr. Wayne Zhou, and Dr. Steve Lambert for valuable comments and discussion.

    FOOTNOTES

* This work was supported by National Institutes of Health Grant GM26701.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. Tel.: 508-856-8988; Fax: 508-856-8987; E-mail: Richard.vallee{at}ummed.edu.

2 R. J. Vasquez and R. B. Vallee, unpublished observations.

    ABBREVIATIONS

The abbreviations used are: aa, amino acid(s); TFE, trifluoroethanol; PH, pleckstrin homology; HA, hemagglutinin.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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