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. 2015 Dec 23;4:e09580. doi: 10.7554/eLife.09580

Munc18-1-regulated stage-wise SNARE assembly underlying synaptic exocytosis

Lu Ma 1, Aleksander A Rebane 1,2,3, Guangcan Yang 1,4, Zhiqun Xi 1, Yuhao Kang 1, Ying Gao 1, Yongli Zhang 1,*
Editor: Stephen C Harrison5
PMCID: PMC4744192  PMID: 26701912

Abstract

Synaptic-soluble N-ethylmaleimide-sensitive factor attachment receptor (SNARE) proteins couple their stage-wise folding/assembly to rapid exocytosis of neurotransmitters in a Munc18-1-dependent manner. The functions of the different assembly stages in exocytosis and the role of Munc18-1 in SNARE assembly are not well understood. Using optical tweezers, we observed four distinct stages of assembly in SNARE N-terminal, middle, C-terminal, and linker domains (or NTD, MD, CTD, and LD, respectively). We found that SNARE layer mutations differentially affect SNARE assembly. Comparison of their effects on SNARE assembly and on exocytosis reveals that NTD and CTD are responsible for vesicle docking and fusion, respectively, whereas MD regulates SNARE assembly and fusion. Munc18-1 initiates SNARE assembly and structures t-SNARE C-terminus independent of syntaxin N-terminal regulatory domain (NRD) and stabilizes the half-zippered SNARE complex dependent upon the NRD. Our observations demonstrate distinct functions of SNARE domains whose assembly is intimately chaperoned by Munc18-1.

DOI: http://dx.doi.org/10.7554/eLife.09580.001

Research Organism: None

eLife digest

Plants, animals and other eukaryotes transport many large molecules within their cells inside membrane-bound packages called vesicles. These vesicles can fuse with the membrane of a target compartment in the cell to deliver their contents inside, or fuse with the cell’s membrane to release the contents outside of the cell.

Membrane fusion is carried out by a group of proteins called SNAREs. These proteins are embedded on the membranes of both the vesicle and its target, and they bind to each other to form a tight complex. This complex docks the vesicle to the target and then acts like a “zipper” to pull the two membranes close enough to fuse. The best-studied SNARE proteins act in nerve cells and fuse vesicles to the cell’s membrane in order to release molecules called neurotransmitters. This process is essential for communication between nerve cells, and relies on a protein called Munc18-1. However, it is not well understood how SNARE proteins assemble into the complex and how Munc18-1 regulates this process.

Ma et al. have now used a tool called “optical tweezers” to pull an assembled SNARE complex apart in the laboratory and then observe how it folds and assembles in a step-by-step process. These experiments showed that the complex assembled in four stages and not three as has been reported in previous work. SNARE proteins are made up of four parts called domains, and Ma et al. observed that the N-terminal domains were the first to bind to each other. Next, the binding progressed to the middle domain, then to the C-terminal domain and finally to the linker domain. An intermediate, half-zippered form was also observed.

Ma et al. next analysed each domain in more detail and found that the N-terminal and C-terminal domains drive the docking of vesicles to the target membrane, the middle domain is crucial for assembling the SNARE complex correctly, and all three domains regulate the fusing of the membranes. Further experiments showed that Munc18-1 promoted the assembly of new SNARE complexes and stabilized the half-zippered form, rather than stabilizing the complex after it had fully assembled. This study will provide a new tool to examine many other proteins that regulate SNARE assembly, and a basis to understand the role of SNARE proteins in brain activity.

DOI: http://dx.doi.org/10.7554/eLife.09580.002

Introduction

SNAREs are evolutionarily conserved molecular machines that drive fusion of transport vesicles with their target membranes, thereby transferring materials and information between different cells or cellular compartments (Sudhof and Rothman, 2009; Wickner and Schekman, 2008; Jahn and Fasshauer, 2012). In the cell, SNARE-mediated membrane fusion requires cognate cytoplasmic Sec1p/Munc18 (SM) proteins (Verhage et al., 2000). Mutations in SNARE and SM proteins have been associated with many important human diseases (Sudhof, 2014; Shen et al., 2014; Saitsu et al., 2008; Shen et al., 2015).

Fusion of synaptic vesicles with the pre-synaptic plasma membrane mediates neurotransmitter release at neuronal and neuromuscular junctions (Sudhof and Rothman, 2009). The fusion requires the vesicle-anchored v-SNARE VAMP2 (also called synaptobrevin), the plasma-membrane-associated t-SNAREs syntaxin-1 and SNAP-25 (Figure 1A), and the SM-protein Munc18-1 (Sollner et al., 1993; Verhage et al., 2000; Sudhof, 2014; Rothman, 2014). Extensive evidence suggests that the t- and v-SNAREs first form a partial trans-SNARE complex bridging the two membranes with the assistance of many regulatory proteins, including Munc18-1, synaptotagmin, complexin, and Munc13, which docks the vesicle to the plasma membrane (Xu et al., 1999; Melia et al., 2002; Gao et al., 2012; Sudhof, 2014; Rothman, 2014). Upon the arrival of an action potential and resultant Ca2+ influx, the trans-SNARE complex rapidly zippers to complete its assembly and membrane fusion. However, an alternative model suggests that SNARE assembly only starts after Ca2+ triggering and completes in one step without any intermediates (Jahn and Fasshauer, 2012). The fully assembled SNARE complex forms a stable parallel four-helix bundle (Sutton et al., 1998; Stein et al., 2009) (Figure 1B). The tight SNARE association is mediated by 15 layers of hydrophobic amino acids and a central ionic layer in the core of the bundle (Fasshauer et al., 1998) (Figure 1A). Numerous studies have shown that layer mutations differentially impact synaptic exocytosis, brain functions, and human psychology (Walter et al., 2010; Mohrmann et al., 2010; Shen et al., 2014; Sudhof, 2014). Thus, it is crucial to understand how SNARE assembly dictates stage-wise exocytosis and how SNARE mutations alter the energetics and kinetics of SNARE assembly to cause their observed phenotypes.

Figure 1. Four distinct stages of SNARE assembly.

(A) Sequences and domain structures of SNARE motifs in VAMP2, syntaxin 1A (SX1), and SNAP-25B (SN1 and SN2). The amino acids in different layers are highlighted in yellow, with the corresponding layer numbers and VAMP2 amino acid numbers labeled. The two amino acids in the red rectangle were mutated to cysteine and crosslinked by a disulfide bridge. The layer amino acids mutated in this study are highlighted in red. (B) Diagram of the experimental setup (Gao et al., 2012; Cecconi et al., 2005). Different functional domains of the SNARE complex are indicated, including the N-terminal domain (NTD), the middle domain (MD), the C-terminal domain (CTD), the linker domain (LD), as well as the N-terminal regulatory domain (NRD) in syntaxin. The positions of four bordering layers are indicated by their layer numbers. (C) Force-extension curves (FECs) of a single SNARE complex with or without (-NRD) the NRD obtained by pulling (black) and then relaxing (gray) the complex. The FECs of the two complexes generally overlap but were shifted along x-axis for clarity. The continuous regions of the FECs corresponding to different assembly states (marked by red numbers, see D) were fitted by the worm-like chain model (red lines). The inset shows a close-up view of the region marked by two red dots. Throughout this work, the time-dependent extension and force were mean-filtered using a time window of 5 ms and plotted in the FECs shown, if not otherwise specified. (D) Six different SNARE assembly states. The states are numbered the same throughout the text (in red). Black numbers indicate different layers. The disordered t-SNARE C-terminus (Tc) in all partially zippered and unzipped SNARE complexes is marked by a dashed rectangle in state 4. The NRD minimally affects intrinsic SNARE assembly and is omitted in the SNARE structures depicted here.

DOI: http://dx.doi.org/10.7554/eLife.09580.003

Figure 1.

Figure 1—figure supplement 1. N-terminal amino acid sequences of rat VAMP 2 and syntaxin-1A showing their different crosslinking sites (marked by red or green boxes) in the SNARE complexes tested.

Figure 1—figure supplement 1.

The amino acids in these sites were substituted with cysteine for crosslinking. In construct I, truncated VAMP2 25-92 and syntaxin-1A (187-265) were crosslinked via the short spacer sequences shown, whereas in other constructs, full cytoplasmic VAMP2 (a.a. 1-96) and syntaxin-1A (a.a. 1-265) were used. Rat SNAP-25 molecules used in all these SNARE complexes had their intrinsic cysteine residues mutated to serine residues. The green box marks the crosslinking site in construct VI used in most of the studies in this work (Figure 1B).

Figure 1—figure supplement 2. Force-extension curves (FECs) of the SNARE complexes crosslinked at different sites shown in Figure 1—figure supplement 1.

Figure 1—figure supplement 2.

All SNARE complexes show similar fast and reversible transitions in the linker domain (LD, red dashed ovals) and in the C-terminal domain (CTD, cyan solid ovals). Whereas constructs I and II exhibit NTD unfolding at high forces (black arrows) and SNARE reassembly at low forces (red arrows), other constructs (III, IV, and V) generally do not crosslink well at the N-terminal sites, leading to tether rupture upon NTD dissociation. NTD, N-terminal domain.

Figure 1—figure supplement 3. FECs of the SNARE complex showing reversible and irreversible transitions and effects of crosslinking near the -6 layer.

Figure 1—figure supplement 3.

The comparison of FEC #1 and FEC #2 reveals that the LD and CTD transitions were not affected by the crosslinking. The SNARE transitions were completely reversible if the SNARE complex was relaxed before the t-SNARE complex was unfolded (FEC #2), as is indicated by overlapping FECs obtained by pulling (green) and then relaxing (red) the SNARE complex. However, after t-SNARE unfolding (black arrow) the same SNARE complex failed to reassemble when relaxed to a force down to 1 pN (FEC #3). CTD, C-terminal domain; FECs, force-extension curves; LD, linker domain. 

Figure 1—figure supplement 4. FECs of a single SNARE complex obtained in the presence 15 µM SNAP-25 in the solution showed that SNAP-25 was required for SNARE assembly.

Figure 1—figure supplement 4.

A single SNARE complex was pulled to high force (FEC in black) to unfold the t-SNARE complex at ~18 pN (rip indicated by the blue arrow) and then relaxed to a low force (FEC in cyan) to observe SNARE re-assembly (red arrow). FECs, force-extension curves.

Figure 1—figure supplement 5. Time-dependent extension (top), instantaneous force (middle), and trap separation (bottom) of the SNARE construct VI (green) or I (black) as the SNARE complex was being pulled by increasing the trap separation at a speed of 10 nm/s.

Figure 1—figure supplement 5.

The different SNARE folding states are marked by red dashed lines and their corresponding state numbers (Figure 1D): 2, the LD-unfolded state; 3, the CTD-unfolded state; 4, the MD-unfolded state; and 5, the NTD-unfolded state. Traces shown here are mean-filtered to 1000 Hz. CTD, C-terminal domain; LD, linker domain; MD, middle domain; NTD, N-terminal domain.

The molecular mechanism by which Munc18-1 regulates SNARE assembly, although essential for membrane fusion, has long been a matter of debate (Rizo and Sudhof, 2012). On one hand, Munc18-1 can significantly enhance the rate and specificity of SNARE-mediated membrane fusion under certain conditions (Shen et al., 2007; Rathore et al., 2010; Yu et al., 2015). On the other hand, Munc18-1 tightly associates with syntaxin in a closed conformation that inhibits SNARE assembly (Colbert et al., 2013; Burkhardt et al., 2008; Dulubova et al., 1999). Munc18-1 also binds with over micromolar affinities to the t-SNARE complex (Zhang et al., 2015), VAMP2 (Parisotto et al., 2014; Xu et al., 2010b), and the ternary SNARE complex (Dulubova et al., 2007; Shen et al., 2007; Rathore et al., 2010). The exact functions of these associations in SNARE assembly and membrane fusion are not well understood (Shen et al., 2007; Burkhardt et al., 2008; Zhou et al., 2013).

SNAREs couple their exergonic folding to membrane fusion (Sudhof and Rothman, 2009; Rothman, 2014). Such a thermodynamic coupling mechanism predicts that any perturbation in SNARE assembly impacts membrane fusion. Significant progresses have been made to test the prediction in the past two decades (Chen et al., 1999; Walter et al., 2010; Mohrmann et al., 2010). However, a quantitative test requires accurate and comprehensive measurements of both the energies and kinetics of SNARE assembly and the rates of membrane fusion for wild-type and various mutant SNARE complexes. Whereas SNARE-mediated membrane fusion has been widely examined in vitro and in vivo, the energetics and kinetics of SNARE assembly have not been well characterized using traditional experimental approaches (Fasshauer et al., 2002; Wiederhold and Fasshauer, 2009). Consequently, a quantitative Munc18-1-dependent model linking the thermodynamics of SNARE assembly to membrane fusion is lacking. For example, although VAMP2 layer mutation F77A abolished exocytosis, isothermal titration calorimetry (ITC) measurements showed that the mutation barely changed SNARE folding energy (Walter et al., 2010). To address this challenge, we have recently established a single-molecule assay for SNARE assembly based on high-resolution optical tweezers and characterized the folding intermediates, energies, and kinetics of four representative SNARE complexes (Gao et al., 2012; Zorman et al., 2014). We have found that all the SNARE complexes are similarly unzipped in two reversible steps and one irreversible step, corresponding to sequential disassembly of SNARE LD, CTD, and NTD at increasing forces. However, complete stage-wise assembly has not directly been observed, due to the slow NTD association. Here, we developed a new SNARE construct that allowed us to measure reversible SNARE assembly and disassembly in four distinct stages and to determine their folding energies and kinetics (Figure 1B). We found that these different assembly stages are regulated by Munc18-1 and play distinct roles in membrane fusion.

Results

Single-molecule manipulation of the SNARE complex

We previously studied a truncated cytoplasmic domain of the synaptic SNARE complex lacking the N-terminal regulatory domain (NRD) of syntaxin (Gao et al., 2012). The NRD contains a ~15 amino acid (a.a.) N-terminal peptide (N-peptide) and a C-terminal Habc domain in a three-helix bundle conformation (Fernandez et al., 1998) (Figure 1B). To observe reversible and regulatory SNARE assembly, we designed SNARE complexes containing the full cytoplasmic domain and an N-terminal crosslinking site between syntaxin and VAMP2. We examined six such SNARE constructs crosslinked at different sites (Figure 1—figure supplements 1,2) and found that the construct crosslinked near the -6 hydrophobic layer exhibited fast and reversible NTD folding/unfolding transition (Figure 1A,B,C). Compared to the slow and irreversible NTD association detected for the SNARE constructs crosslinked N-terminal to the -7 layer (Gao et al., 2012) (Figure 1—figure supplements 12, construct I), the fast NTD folding observed here implicated the existence of a nucleation site for NTD zippering near or N-terminal to the -6 layer. This new construct was used for most of the experiments described below. To manipulate a single SNARE complex, we either pulled or relaxed the complex by moving one optical trap relative to the other at a speed of 10 nm/s or held the complex under constant average force at a fixed trap separation (Figure 1B). Both force and extension of the protein-DNA tether were recorded at 10 kHz and used to derive the conformational and energetic changes of the SNARE complex in real time (Gao et al., 2012). Specifically, for a reversible two-state transition, the folding energy of the associated protein domain can be measured based on the mechanical work required to unfold the domain, which is equal to the equilibrium force multiplied by the extension change related to the transition (Bustamante et al., 2004; Liphardt et al., 2001; Gao et al., 2011).

Four stages of SNARE assembly in four domains

The force-extension curves (FECs) obtained by pulling and then relaxing a single SNARE complex (Figure 1C) showed four reversible transitions with fast extension flickering (among states 1 to 5) and one irreversible unfolding transition (from states 5 to 6), indicating cooperative unfolding/refolding of five SNARE domains (Video 1). These discrete transitions were separated by continuous regions caused by elastic response of the SNARE-DNA tether to force change, while the SNARE complex remained in the same folding state. Accordingly, these FEC regions could be fit by a worm-like chain model for both the DNA handle and the unfolded polypeptide (Bustamante et al., 1994; Marko and Siggia, 1995). The fitting of these regions yielded different contour lengths for the polypeptide unfolded in the SNARE complex, which were used to derive the structures of SNARE assembly intermediates (Figure 1D). The FECs associated with states 1–3 were identical to the FECs previously reported (Gao et al., 2012) and independent of the N-terminal crosslinking (Figure 1—figure supplement 2,3). The comparison suggests that the states 1, 2, and 3 are the fully folded, the LD-unfolded, and the partially-zippered SNARE complexes, respectively (Figure 1D). A new reversible NTD transition partly overlapped the CTD transition (between states 3 and 5, Figure 1C, inset). Relaxing the complex from state 5 led to a FEC that overlaps the FEC in the pulling phase, indicating complete and reversible reassembly of the SNARE complex (Figure 1—figure supplement 3). However, pulling the complex in state 5 to higher forces saw a small rip resulting from unfolding of the remaining t-SNARE complex (from state 5 to state 6) (Gao et al., 2012) (Figure 1C,D). No additional unfolding event was observed when further pulling the complex in state 6 (Figure 1—figure supplement 3, #3), indicating that the SNARE complex was fully disassembled. We then relaxed the molecule to a force of 1 pN to check if SNARE reassembled. Unexpectedly, no single SNARE re-assembly event was detected among 45 different SNARE complexes tested. Consistent with our previous observation (Gao et al., 2012), the failure of reassembly was caused by dissociation of the SNAP-25 molecule upon t-SNARE unfolding, because adding 15 µM SNAP-25 into the solution rescued the assembly (Figure 1—figure supplement 4).

Video 1. Optical tweezers manipulate a single SNARE complex to reveal its folding intermediates, energetics, and kinetics.

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DOI: 10.7554/eLife.09580.009

Not drawn to scale. Note that the single-SNARE complex was being pulled or relaxed by moving the optical trap on the right (not shown) at a speed of 10 nm/s. The tension and extension of the DNA-protein tether was monitored to derive the conformations, energetics, and kinetics of SNARE assembly.

DOI: http://dx.doi.org/10.7554/eLife.09580.009

Close inspection shows an additional state hidden in the NTD transition, state 4 (Figure 1—figure supplement 5). This state had a maximum lifetime of ~1 ms and rapidly transited between state 3 and state 5 (Figure 2A and Figure 2—figure supplement 1). This transition was clearly seen in some FECs and extension traces plotted at ≥1 kHz bandwidth (Figure 2A) and was also found in our previous measurements (Gao et al., 2012) (Figure 1—figure supplement 5). Based on the measured extension changes accompanying the state transitions and the well-defined structures of the initial and final states of SNARE assembly (states 1 and 6), we derived the intermediate conformations (Figure 1D and 'Materials and methods'). In the partially-zippered state 3, the VAMP2 CTD and the t-SNARE CTD are unfolded from layer +8 to layer +3 and layer +5, respectively, whereas the remainder of the SNAREs are largely helical as in the four-helix bundle. This structure is consistent with that of a different trans-SNARE complex located on the yeast vacuole (Schwartz and Merz, 2009). In the MD-unfolded state 4, VAMP2 is unfolded further to the ionic layer. Therefore, the MD consists of the ionic layer (0 layer) and the +1 and +2 layers exclusively comprising leucine and isoleucine residues known to form strong coiled coils (Figure 1A), which leads to the higher mechanical stability of the MD than the CTD and their distinct transitions. In the unzipped SNARE state 5, the t-SNARE complex remains in a three-helix bundle conformation, but with a frayed C-terminus (Tc). These conformations were further corroborated by results of protein binding and SNARE mutations described below.

Figure 2. Energetics and kinetics of SNARE assembly.

(A) Extension-time trajectories of a single SNARE complex under the indicated constant mean forces. The idealized state transitions derived from hidden-Markov modeling (HMM) are shown as red lines. The positions of different states (red numbers) are marked by green dashed lines. Data were mean-filtered using a time window of 0.2 ms and shown. (B) Probability density distributions of the extensions corresponding to the first three traces in A and their best fits by a sum of four Gaussian functions (lines). (C) HMM-derived state populations (upper panel, symbols) and transition rates (lower panel, symbols) are shown as a function of the mean forces. The unfolding and folding rates are shown as solid and hollow symbols, respectively. Their best model fits are shown as lines (‘Materials and methods’). (D) Simplified folding energy landscapes of the wild-type (WT) and the mutant (L60A) SNARE complexes. The abscissa denotes the VAMP2 residue number bordering the structured and unstructured polypeptide regions in the corresponding folding state. All stable states (solid) and transition states (hollow) are defined in the presence of forces.

DOI: http://dx.doi.org/10.7554/eLife.09580.010

Figure 2.

Figure 2—figure supplement 1. Force-dependent average lifetimes of the four states 2–5 involved in the SNARE assembly (symbols) and their best fits (lines).

Figure 2—figure supplement 1.

See ‘Materials and methods’ for details.
Figure 2—figure supplement 2. Transition rates determined by hidden-Markov modeling (HMM) shows that the t- and v-SNAREs sequentially assemble like a molecular zipper.

Figure 2—figure supplement 2.

The rates of non-sequential transitions were negligible compared to those of sequential transitions.
Figure 2—figure supplement 3. Modeling SNARE assembly observed in optical traps using the crystal structure of the SNARE complex and a simplified energy landscape.

Figure 2—figure supplement 3.

The total extension of the protein-DNA tether and the total energy of detection system could be calculated from the model and fit to the experimental measurements to derive the folding energies and kinetics of the SNARE complex at zero force (see ‘Materials and methods’ for details).

In conclusion, we identified an independent SNARE folding domain, the middle domain, and observed that the SNARE complex zippers in four distinct and sequential stages from NTD to MD to CTD and finally to LD. These results clarify the partially zippered SNARE states previously derived (Schwartz and Merz, 2009; Gao et al., 2012; Min et al., 2013).

Energetics and kinetics of SNARE assembly

To better characterize the intermediates and their associated energies and transition kinetics, we measured the extension-time trajectories of the SNARE complex at different constant mean forces. Simultaneous transitions among four states 2–5 could be resolved (Figure 2A and Video 2). The positions, populations, transition rates, and lifetimes (Figure 2—figure supplement 1) associated with these states could be determined by hidden-Markov modeling (HMM) (McKinney et al., 2006; Gao et al., 2011; Rebane, et al., 2016). Accordingly, the probability density distributions of the extensions were fit well by a sum of four Gaussian functions (Figure 2B), confirming the four-state transitions and revealing the average state positions and populations consistent with those derived from HMM. Figure 2C shows populations of the four states (top panel) and rates of the main transitions among these states (bottom panel), measured on a single representative SNARE complex. The transitions are approximately sequential, because the rates for sequential transitions are over two orders of magnitude greater than the rates for non-sequential transitions (Figure 2—figure supplement 2).

Video 2. Force-induced SNARE folding and unfolding transitions under thermodynamic equilibrium among four distinct states.

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DOI: 10.7554/eLife.09580.014

The single SNARE complex was held at the indicated mean force at a constant trap separation. The stochastic unfolding and refolding transitions of the SNARE complex represent its thermodynamic fluctuations when the free energies of the four states become close (<5 kBT) in the presence of force (Liphardt et al., 2001).

DOI: http://dx.doi.org/10.7554/eLife.09580.014

We developed a nonlinear model to describe protein transitions in optical traps (Rebane, et al., 2016; Gao et al., 2012; Xi et al., 2012) (Figure 2—figure supplement 3 and 'Materials and methods'). We modeled SNARE zippering as VAMP2 folding along a t-SNARE template based on the crystal structure of the SNARE complex. The model included the extension and energy contributions of both the folded and unfolded portions of the complex along the pulling direction. In addition, we calculated the populations of different folding states and their transition rates based on the model. Simultaneous nonlinear least-squares fitting of the calculations to the corresponding measurements yielded the conformations (Figure 1D) and energies of the three intermediate states and their associated transition states at zero force, resulting in the simplified energy landscape of SNARE folding/assembly (Figure 2D). Specifically, the folding energies of NTD, MD, and CTD are 25 (±2, S.D.) kBT, 13 (±1) kBT, and 22 (±3) kBT, respectively, where kB is the Boltzmann constant and T= 296 K the room temperature, with kBT=0.59 kcal/mol. Thus, the SNARE complex has total zippering energy of 68 (±4) kBT, including 8 (±2) kBT LD folding energy (Gao et al., 2012). Folding of the NTD and CTD is downhill. In contrast, the MD has a folding energy barrier of 5.0 (±0.6) kBT located close to the ionic layer, indicating a high-energy penalty to dehydrate the ionic layer for MD assembly (Rebane, et al., 2016).

Vc peptide induces folding of t-SNARE C-terminus and attenuates SNARE zippering

A distinct feature of our derived conformations is a frayed Tc in states 3–5 (Figure 1D). To confirm the disordered Tc, we repeated the above experiments by adding a peptide comprising the C-terminal sequence 49–96 or layers from −2 to +8 of VAMP2 (Vc peptide) to the solution (Figure 1A). We predicted that binding of the Vc peptide to the t-SNARE complex would induce a coil-to-helix transition in Tc and inhibit or attenuate SNARE zippering into the two partially-zippered states 3 and 4. The Vc peptide is widely used to facilitate studies of SNARE-mediated fusion (Melia et al., 2002; Pobbati et al., 2006; Hernandez et al., 2012). Pre-bound to the t-SNARE complex, this peptide greatly enhances membrane fusion, probably because the Vc peptide stabilizes the t-SNARE complex in a conformation ready to pair with VAMP2, and thus helping to initiate SNARE zippering (Pobbati et al., 2006). In the presence of 44 μM Vc peptide in the solution, we found that the Vc peptide frequently bound to the SNARE complex. The binding was manifested by a sudden SNARE transition into new Vc-bound states (cyan region in Figure 3A,B). Correspondingly, the binding caused a dramatic change in the histogram distribution of the extension (Figure 3C). Once bound, the Vc peptide did not dissociate from the SNARE complex, indicating that the Vc peptide outcompeted the VAMP2 molecule to tightly associate with the t-SNARE complex under our experimental conditions. The lifetime of the Vc-bound states was estimated to be greater than 10 min in the force range of NTD and CTD transitions. The Vc-bound SNARE states have a unimodal extension distribution (Figure 3C), whose peak extension is 2.7 nm less than the average extension of the NTD-unfolded state 5, with an average shortening of 2.3 (±0.5, N=8) nm (Figure 3D). The extension shortening upon Vc binding is consistent with the predicted coil-to-helix transition in Tc, confirming the disordered Tc. The comparison of the extension distributions also reveals that the Vc peptide predominantly stabilized the SNARE complex in the Vn-unfolded state (state 8) (Figure 3C). Partially zippered states were only transient, indicated by downward extension excursions to a new state (state 7) with its extension greater than those of the partially zippered states 3 and 4. Thus, upon binding to the t-SNARE complex, the Vc peptide acted as a roadblock to attenuate VAMP2 from zippering. However, the Vc peptide was displaced by the VAMP2 molecule at an average force of 6 (± 1) pN upon relaxation. Taken together, these observations supported the conformations of the partially zippered states and the unzipped state derived by us (Figure 1D) and indicated that the Vc peptide strongly attenuated SNARE zippering.

Figure 3. Vc peptide induces a coil-to-helix transition in the t-SNARE C-terminus (Tc).

Figure 3.

(A) Extension-time trajectory showing changes in SNARE folding kinetics caused by binding of the Vc peptide to the t-SNARE in the SNARE complex. The Vc-bound region is colored in cyan. The positions of different states are marked by red dashed lines and the corresponding state numbers. Data were filtered using a time window of 1 ms. (B) Close-up view of the region in A marked by a rectangle. Data were filtered using a time window of 0.6 ms. (C) Probability density distributions of the extensions in A before (black) and after (cyan) Vc binding. (D) Diagram illustrating the Vc-induced conformational transitions. The extension changes averaged over eight Vc-binding events are indicated.

DOI: http://dx.doi.org/10.7554/eLife.09580.015

Position-dependent effects of layer mutation on SNARE assembly

To understand functions of the different stages of SNARE assembly in membrane fusion and exocytosis, we measured the folding energies and kinetics of 15 SNARE complexes mutated in each layer from −5 to +8. Their effects on exocytosis will be discussed in the forthcoming section. Most of these mutations are alanine substitutions in VAMP2 (Walter et al., 2010) (Figure 1A). Three other mutations are VAMP2 A67S, SNAP-25 M71A/I192A (Mohrmann et al., 2010), and syntaxin T251I (Lagow et al., 2007). These mutations were expected to mainly perturb SNARE zippering but minimally interfere with binding of regulatory proteins to SNARE proteins, which allows us to focus on the effect of intrinsic SNARE assembly on exocytosis. Furthermore, most of the mutants have been characterized in vivo for their impacts in exocytosis and neurotransmitter release (Walter et al., 2010; Mohrmann et al., 2010; Lagow et al., 2007). Related mutations have been associated with many neurological disorders in humans (Shen et al., 2014; Rohena et al., 2013).

All SNARE complexes containing single alanine substitutions in the NTD, except for M46A, exhibit similar FECs and transition kinetics as the wild-type (Figures 46 and Figure 5—figure supplement 1). Therefore, single alanine substitutions in the NTD generally have minor impact on SNARE assembly. In contrast, M46A reduced the stability of NTD, as is indicated by a small decrease in the force for NTD transition compared to the wild-type (Figures 4 and 6). The approximately equal mechanical stabilities of MD and NTD now led to disappearance of the intermediate state 4 (Figure 5). Consequently, both MD and NTD transited cooperatively as one unit (designated as MD_NTD) between the CTD-unfolded state 3 and the unzipped state 5 (Figure 4—figure supplement 1), in contrast with the sequential MD and NTD transitions (designated as MD+NTD) seen for the wild-type SNARE complex (Figure 2A). Thus, M46A altered SNARE assembly kinetics and pathway. Finally, the double mutation V39A/V42A dramatically decreased the folding rate of NTD (Figure 5). In addition, it destabilized NTD by 3 kBT (Figure 7).

Figure 4. Position-dependent effects of layer mutations on SNARE assembly shown by the FECs of the wild-type and mutant SNARE complexes.

The SNARE mutations and their layer numbers are colored based on their associated domains: blue for NTD, green for MD, and red for CTD. While most mutants assemble sequentially as the wild type (WT), some mutants exhibit altered folding pathways, in which two neighboring domains fold and unfold cooperatively as combined domains. Throughout the text, two-state transitions of these new domains are marked by their associated subdomains connected by “_” (Figure 4—figure supplement 1). By comparison, overlapping sequential transitions are indicated by their associated domains linked by “+”. Different folding domains are marked by unique colored ovals or rectangles. Folding energies of the same domain in different SNARE complexes can be compared by the equilibrium forces of the domain transition. The black and gray horizontal lines indicate the average equilibrium forces of CTD (16.5 ± 0.8 pN) and MD+NTD (17.2 ± 0.8 pN), respectively, of the wild-type SNARE complex. CTD, C-terminal domain; FECs, Force-extensioncurves; MD, middle domain; NTD, N-terminal domain.

DOI: http://dx.doi.org/10.7554/eLife.09580.016

Figure 4.

Figure 4—figure supplement 1. Comparison of sequential and cooperative domain transitions, using MD and NTD as an example.

Figure 4—figure supplement 1.

The wild type SNARE complex sequentially unfolds in the order of LD, CTD, MD, and NTD and folds in the reverse order, which is caused by the increasing mechanical stabilities of domains from LD to NTD. However, a SNARE mutation may preferentially alter the mechanical stability of the domain in which the mutation resides, changing the order of the domain stabilities. As a consequence, we found that the SNARE mutations often led to combinations of two neighboring domains into new domains that cooperatively folded and unfolded as single units. Throughout the text, these new domains are designated by their associated sub-domains linked by “_”. All neighboring domain combinations were observed, including LD_CTD in SNAP-25 mutant M71A/I192A (Figures 4 and 6), CTD_MD in VAMP2 mutants L60A and L63, and MD_NTD in VAMP2 mutant M46A (Figures 4 and 5). By comparison, two or more sequential transitions in an overlapping force region are designed by their associated domains linked by “+”. For example, the transitions shown in Figure 2A can be indicated by “CTD+MD+NTD”. CTD, C-terminal domain; LD, linker domain; MD, middle domain; NTD, N-terminal domain.

Figure 6. Comparison of force-dependent state populations and transition rates of the mutant SNARE complexes.

Figure 6.

Experimental measurements from representative single SNARE complexes (symbols) were fit by a simplified energy landscape model of SNARE assembly (lines) to derive the folding energies of different domains (‘Materials and methods’).

DOI: http://dx.doi.org/10.7554/eLife.09580.021

Figure 5. Extension-time trajectories of the mutant SNARE complexes under constant forces showing effects of mutations on the transition kinetics of different SNARE domains.

(A) Extension-time trajectories. The domains involved in the observed transitions and the mean forces (F) are indicated following the colored mutation names in bold (Figure 4—figure supplement 1). Positions of different states are marked by green dashed lines. (B) Probability density distributions of the extensions under the indicated constant forces (symbols) revealing structural changes in the intermediates of SNARE assembly. The distributions could be fitted by 2-4 Gaussian functions (solid lines), and were horizontally shifted to align the peaks corresponding to different states (indicated by the vertical shaded bars).

DOI: http://dx.doi.org/10.7554/eLife.09580.018

Figure 5.

Figure 5—figure supplement 1. Extension-time trajectories of mutant SNARE complexes showing indicated domain transitions under constant mean forces.

Figure 5—figure supplement 1.

Data were mean-filtered using a time window of 1 ms and plotted.
Figure 5—figure supplement 2. Probability density distributions of the extensions of the mutant SNARE complex R56A under different constant mean forces.

Figure 5—figure supplement 2.

The distributions were calculated using the best-fit parameters from the HMM analysis of the extension trajectories, which were filtered using a time window of 0.2 ms. A four-state SNARE transition is seen from the distributions. HMM, hidden-Markov modeling.

Figure 7. Layer mutations differentially affect folding energies and pathways of SNARE assembly.

Figure 7.

The wild-type and most mutant SNARE complexes assemble sequentially in the order of NTD, MD, CTD, and LD, with their total MD and NTD (MD+NTD) energies and CTD energies shown in black and gray bars, respectively. The energies of CTD and MD+NTD of the wild-type SNARE complex are marked by black and gray lines, respectively. Other mutants contain cooperative transitions involving two domains (Figure 4—figure supplement 1), which are indicated by colored bars. The double mutations in the +5 layer in SNAP-25 cause cooperative LD and CTD transition, but only the CTD energy is shown for better comparison, assuming an LD folding energy of 8 kBT (Gao et al., 2012). The mutant amino acids and their layer numbers that impair or enhance exocytosis are colored in red or green, respectively. Error bars represent standard deviations of the measurement. CTD, C-terminal domain; LD, linker domain; MD, middle domain; NTD, N-terminal domain.

DOI: http://dx.doi.org/10.7554/eLife.09580.022

Three point mutations in MD caused great changes in SNARE zippering. First, R56A destabilized both NTD and CTD (Figures 4 and 7), indicating that the ionic layer globally stabilizes the SNARE complex (Rebane, et al., 2016). In addition, R56A increased the extension change associated with the MD transition (Figure 5 and Figure 5—figure supplement 2), corroborating the independent MD transition and the N-terminal border position of R56 in the MD. In contrast, L60A (+1) and L63A (+2) abolished the independent MD transition and caused MD to merge with CTD (Figure 5). Consequently, the combined CTD and MD (CTD_MD) transited cooperatively as a distinct domain with an average extension change approximately equal to the sum (~11 nm) of the extension changes for the CTD (6–7 nm) and the MD (3–4 nm). Therefore, mutations at +1 and +2 layers altered the pathway of SNARE assembly, in which the distinct MD assembly was bypassed. Accordingly, all MD mutations abolished the energy barrier in MD folding (Rebane, et al., 2016) (Figure 2D). Finally, we found that all MD mutants frequently and abruptly switched their transition kinetics (Figure 8), indicating an important role of MD in accurate and robust SNARE assembly. Because of the abundant heterogeneity, the folding energies of the MD mutants were only measured from the canonical regions. In summary, the middle domain plays a pivotal role in robust and correct stage-wise SNARE assembly, and its mutation leads to changes in SNARE assembly pathway and accuracy.

Figure 8. Extension-time trajectories showing kinetic heterogeneity in SNARE folding due to MD Layer Mutation.

Figure 8.

The canonical (occurring more frequently) and the altered transitions are shown in black and red, respectively. The heterogeneity in SNARE assembly was manifested by abrupt changes in transition rates and state populations. Some of these kinetic switching events (a and c) were reversible in our experimental time scale (typically <30 min), indicating that the kinetic heterogeneity was caused neither by impurities in our SNARE constructs nor by photodamage of SNARE proteins in optical traps. However, the underlying molecular mechanism for such heterogeneity is unknown, but likely related to the metastable t-SNARE complex.

DOI: http://dx.doi.org/10.7554/eLife.09580.023

The CTD layer mutations affected CTD and LD folding in a position-dependent manner, but did not alter NTD folding. The two mutations A67S (+3) and L84A (+8) at the borders of the CTD had only minor effects on SNARE assembly (Figures 4, 7, and Figure 5—figure supplement 1). In contrast, L70A (+4) and F77A (+6) in VAMP2 and M71A/I192A (+5) in SNAP-25 greatly reduced the force ranges of the CTD transition that now overlapped the LD transition. In particular, the +6 layer mutation weakened both CTD and LD (Figures 4,6,7, and Figure 5—figure supplement 1). Correspondingly, alanine substitutions at +4, +5 and +6 layers dramatically decreased CTD folding energies by 10 kBT, 13 kBT, and 12 kBT, respectively, compared to the wild-type. Our energy measurement of F77A contrasts with the previous measurement by ITC and is consistent with its ablation of exocytosis (Walter et al., 2010). The syntaxin mutation T251I (+7) is unusual, because it increased the CTD zippering energy by 5 kBT (Figures 4 and 7), quantitatively confirming the previous inference based on structural modeling (Lagow et al., 2007). Taken together, the CTD stability is sensitive to mutations in layers from +4 to +7.

In summary, the effects of layer mutations on SNARE assembly strongly depend on their positions, ranging from minimal perturbation to significant changes in the energetics, intermediates, or kinetics of SNARE assembly.

Munc18-1 promotes de novo SNARE assembly

To examine effects of Munc18-1 on SNARE assembly, we added 2–50 µM Munc18-1 into the solution where a single SNARE complex (Figure 1B) was being pulled in a microfluidic chamber (Zhang et al., 2012). We observed three force-dependent activities of Munc18-1 in SNARE assembly, consistent with the previously reported multiple modes of binding between Munc18-1 and the SNARE complex (Sudhof and Rothman, 2009; Sudhof, 2014).

The most distinct Munc18-1 activity is to enhance de novo SNARE assembly. To observe this activity, we completely unfolded the SNARE complex and then relaxed the complex to a low force to detect its possible reassembly (Figure 9A). In the absence of Munc18-1, no SNARE reassembly was observed (Figure 1C and 9B) due to dissociation of the SNAP-25 molecule (Figure 1—figure supplement 4). In contrast, in the presence of 10 µM Munc18-1, 45% of 113 completely unfolded SNARE complexes showed full reassembly (Figure 9A,B). This observation suggests that Munc18-1 held the SNAP-25 molecule together with the tethered syntaxin or VAMP2 as t-SNARE unfolded, facilitating de novo SNARE assembly. The SNARE assembly occurred in a force range of 1-16 pN, with an average force of 8.5 pN (Figure 9C). In addition, the assembly events tended to appear in consecutive rounds of pulling and relaxing the same SNARE complex (Figure 9A, #3-#5). Although the probability to observe a SNARE reassembly event was 0.45 under our experimental conditions, the probability to detect a SNARE reassembly event after another was 0.8, suggesting a strong correlation between the different reassembly events mediated by Munc18-1. An appealing interpretation for the correlation is that the same Munc18-1 molecule mediated the consecutive reassembly events without dissociation from the SNARE complex during its multiple rounds of disassembly and reassembly. The Munc18-1-mediated SNARE assembly was not abolished by the two VAMP2 layer mutations L60A and L63A (Figure 9B). This finding suggests that, despite their effect on the accuracy of intrinsic SNARE assembly, neither MD mutation significantly affect Munc18-1-dependent de novo SNARE assembly. Finally, we found that Munc18-1 similarly promoted SNARE assembly (Figure 9D) when the SNARE complex was crosslinked at a site N-terminal to the SNARE bundle (Construct I in Figure 1—figure supplement 1), indicating that the Munc18-1 activity was not caused by specific SNARE crosslinking. Interestingly, in this case, SNARE assembly occurred in two steps: t-SNARE formation at 12-17 pN, followed by cooperative SNARE zippering at 5-10 pN. Thus, Munc18-1 may mediate de novo SNARE assembly via a t-SNARE intermediate.

Figure 9. Munc18-1 helps to initiate SNARE assembly.

Figure 9.

(A) FECs of single SNARE complexes obtained in the presence of 10 µM Munc18-1 in the solution. Black and red arrows indicate t-SNARE unfolding and de novo SNARE reassembly, respectively. The FECs #3-#5 were obtained by consecutively pulling and relaxing the same SNARE complex. (B) Percentage of de novo assembly (%) among a total number of unfolded SNARE complexes tested (N) for the wild-type (WT), NRD-removed (-NRD), and mutant (L60A and L63A) SNARE complexes in the presence (+) or absence (−) of 10 µM Munc18-1. (C) Histogram distributions of the forces associated with the Munc18-1-mediated de novoSNARE assembly. (D) FECs of the SNARE complexes crosslinked at a site N-terminal to the SNARE motifs (Figure 1—figure supplement 1, construct I) in the absence (−Munc18-1) or presence (+Munc18-1) of Munc18-1. In the absence of Munc18-1, SNAP-25 tended to dissociate from the tethered syntaxin and VAMP2 when the t-SNARE complex was unfolded (black arrows). As a result, the SNARE complex generally reassembled for no more than four rounds during repetitive pulling and relaxation (Gao et al., 2012). However, in the presence of 10 µM Munc18-1, the yield of SNARE reassembly was greatly enhanced, leading to robust SNARE disassembly and reassembly for at least 19 rounds on the single SNARE complex. For clarity, only the FECs of some rounds of pulling and relaxation (indicated by the red numbers) are shown. In this case, full SNARE reassembly (red arrows) was preceded by t-SNARE formation (blue arrows) in the force range of 12-17 pN, due to the slow and force-sensitive NTD assembly of this construct. FECs, force-extension curves; NTD, N-terminal domain.

DOI: http://dx.doi.org/10.7554/eLife.09580.024

Munc18-1 stabilizes the half-zippered SNARE complex

Under constant forces, we observed a series of prominent long-dwelling states in the middle of fast SNARE transitions (Figure 10A,B), revealing a new Munc18-1-dependent state. The state lasted from 0.03 to ~30 s, with an average dwell time of 2.8 s (Figure 10C) and was detected in a force range of 15-19 pN, with an average of 17.1 pN (Figure 10D). The new state has an extension corresponding to VAMP2 unzipped to a position between layers 0 and +1 (Figure 10E), and is thus a half-zippered state (state 9). The occurrence rate of this state was 0.012 s-1 on average measured from a total experimental time of 6908 s. The rate was strongly force-dependent (Figure 10D). As a result, the half-zippered state was not found in the force range below 15 pN.

Figure 10. Munc18-1 stabilizes the half-zippered SNARE complex.

Figure 10.

(A–B) Extension-time trajectories of single wild-type or mutant (L70A) SNARE complexes under constant forces in the presence of 10 µM Munc18-1 in the solution. The red regions indicate the Munc18-1-bound state (state 9). A close-up view of the region in the dashed rectangle in i is shown in (B), iv. (C) Histogram distribution of the dwell times of the Munc18-1-stabilized half-zippered state. (D) Histogram distribution of the forces of the Munc18-1-stabilized half-zippered state. (E) Probability density distributions of the extensions of the Munc18-1-unbound states (black) and the Munc18-1-bound state (red) calculated from the corresponding regions in trace ii in A. Different peaks represent different SNARE folding states numbered as in Figure 1D.

DOI: http://dx.doi.org/10.7554/eLife.09580.025

To stabilize the SNARE complex in a half-zippered state, Munc18-1 needs to stabilize NTD and to destabilize CTD. As a step to pinpoint the mechanism, we repeated the above experiment using the SNARE complex containing the VAMP2 mutation L70A. We found that L70A did not significantly affect the Munc18-1-stabilized half-zippered state (Figure 10A, iii), implying that Munc18-1 did not strongly interact with L70 in this observed Munc18-1 activity. Instead, Munc18-1 might partly bind the C-terminal domain of the t-SNARE in the SNARE complex to attenuate CTD zippering.

In conclusion, Munc18-1 stabilized the half-zippered SNARE complex in a force-dependent manner. Because the trans-SNARE complex is likely half-zippered (Gao et al., 2012; Kyoung et al., 2011; Min et al., 2013; Li et al., 2014), our observation corroborates that Munc18-1 enhances assembly of trans-SNARE complexes to promote membrane fusion (Shen et al., 2007; Rathore et al., 2010).

Munc18-1 requires NRD to stabilize the half-zippered SNARE complex

Previous experiments show that Munc18-1 requires the NRD to enhance membrane fusion in vitro and exocytosis in vivo (Shen et al., 2007; Dulubova et al., 2007; Zhou et al., 2013). Specifically, Munc18-1 is recruited by the N-peptide in the NRD to bind trans-SNARE complexes (Shen et al., 2010). Interestingly, once Munc18-1 associates with trans-SNARE complexes, the NRD becomes dispensable for subsequent membrane fusion (Rathore et al., 2010). These findings suggest that Munc18-1 binds SNARE complexes in both NRD-dependent and NRD-independent modes and can dynamically transit between the two binding modes (Hu et al., 2011). To pinpoint the possible role of the NRD in the Munc18-1-dependent SNARE zippering observed by us, we removed the NRD in the SNARE construct (Figure 1B) and repeated the above experiments. The NRD removal did not cause significant changes in the intrinsic stage-wise SNARE assembly (Figure 1C,2A, -NRD), which suggests that the NRD barely interacted with the SNARE motifs. Furthermore, the NRD removal did not alter the de novo SNARE assembly (marked by red arrows in Figure 11A, #1, and 9B), indicating that the NRD is dispensable for this Munc18-1-dependent activity. However, Munc18-1 no longer stabilized the half-zippered state well (Figure 11B,C and Figure 11-figure supplement 1). Instead, Munc18-1 mainly stabilized a novel state (state 11) with a distinct extension that was 1–3.5 nm less than the NTD-unfolded state 5 (Figure 11D and Figure 11-figure supplement 1). The average extension difference between state 11 and state 5 is 2.5 (±0.7, N=16) nm, approximately equal to the extension shortening caused by binding of the Vc peptide (Figure 3D). This Munc18-1 activity occurred at a rate of 0.015 s-1 measured from a total experimental time of 4018 s. Surprisingly, Munc18-1 now bound much more strongly to the SNARE complex. More than half the Munc18-1-bound states lasted more than 30 s. Therefore, the NRD removal significantly enhances the thermodynamic stability of Munc18-1 binding to the SNARE complex.

Figure 11. Munc18-1 stabilizes the half-zippered SNARE complex in an NRD-dependent manner and binds the t-SNARE complex to structure Tc in an NRD-independent manner.

(A) FECs of the SNARE complex lacking the NRD in the presence of 10 µM Munc18-1 in the solution. The rectangle marks the Munc18-1-mediated reversible transition in FEC #2 between states 10 and 11 illustrated in E. The FECs #3-#5 were obtained from the same SNARE complex in three consecutive rounds of pulling and relaxation. The FECs of different rounds overlap well (#3-#5) but are shifted along the x-axis for clarity (#3, #4, and #5). The states corresponding to some regions of FECs are indicated by their corresponding state numbers (Figures 11E and 1D). In FECs #3 and #4 the point of Munc18-1 binding is marked by a green dot. (B–C) Extension-time trajectories of the SNARE complex lacking an NRD under constant forces in the presence of 10 µM Munc18-1. The cyan regions indicate the Munc18-1-bound states (states 10 and 11). A close-up view of the region in B in the dashed rectangle is shown in (C). (D) Probability density distributions of the extensions of the Munc18-1-unbound states (black) and the Munc18-1-bound states (cyan) calculated from the corresponding regions in the trace shown in B. Different peaks represent different SNARE folding states numbered in red as in E and Figure 1D. (E) Diagram illustrating effects of Munc18-1 on assembly of the SNARE complex lacking an NRD and the associated average extension changes of the different states. FECs, force-extension curves; NRD, N-terminal regulatory domain.

DOI: http://dx.doi.org/10.7554/eLife.09580.026

Figure 11.

Figure 11—figure supplement 1. (A–B) Extension-time trajectory of the SNARE complex lacking an NRD in the presence of 10 μM Munc18-1 in the solution.

Figure 11—figure supplement 1.

The regions corresponding to the Munc18-1-bound states are colored cyan. The positions of different states are marked by red dashed lines. A close-up view of the region in (A) marked by a rectangle is shown in (B). (C) Probability density distributions (symbols) of the extensions corresponding to regions in A marked by black and cyan bars without and with Munc18-1 bound. The lines are best-fits of the distributions using a sum of three or one Gaussian function for the Munc18-1-unbound states or Munc18-bound states, respectively. NRD, N-terminal regulatory domain.
Figure 11—figure supplement 2. FECs of the SNARE complexes with the NRD (+NRD) obtained in the absence (−Munc18-1) or presence (+Munc18-1) of 10 µM Munc18-1.

Figure 11—figure supplement 2.

The region marked by a red rectangle shows the Munc18-1-mediated conformational transition between states 10 and 11 illustrated in Figure 11E. The green arrow indicates Munc18-1 displacement and SNARE reassembly. Compared with the FEC of the SNARE complex lacking the NRD (Figure 11A, #2), the results here suggest that even in the presence of the NRD, Munc18-1 could bypass the NRD to bind the SNARE complex in an NRD-independent manner. FECs, force-extension curves; NRD, N-terminal regulatory domain.
Figure 11—figure supplement 3. Extension-time trajectory of the wild-type SNARE complex with the NRD in the presence of 10 μM Munc18-1.

Figure 11—figure supplement 3.

The regions corresponding to the Munc18-1-bound states are colored cyan. The positions of different states are marked by red dashed lines. A close-up view of the region in the top trace marked by a rectangle is shown at the bottom. Compared with the trajectories for the SNARE complex lacking the NRD (Figure 11B,C), the trajectories here demonstrate that Munc18-1 could tightly bind t-SNARE and structure Tc in an NRD-independent manner, even in the presence of the NRD. NRD, N-terminal regulatory domain.

Munc18-1 also induced a minor state (state 10) that reversibly transited with the major state 11 (Figure 11C,D). State 10 had an average extension close to the half-zippered state 9, but with higher stability than state 9. When relaxing the Munc18-1-bound SNARE complex to a lower force, we saw an equilibrium shift from state 11 to state 10, reaching equilibrium at an average force of 14.0 (±1.2) pN with corresponding extension change of 5.7 (±0.6) nm (Figure 11A, #2, region marked by red rectangle). Munc18-1 was displaced from the SNARE complex in state 10 in a force range of 8-13 pN (indicated by the green arrow), with an average force of 10.3 pN. The displacement was accompanied by full SNARE assembly, which was confirmed by the FEC of the subsequent pulling phase. Thus, Munc18-1 attenuated SNARE NTD zippering in the absence of the NRD, although Munc18-1 stabilized the NTD in state 9 in the presence of the NRD. Because state 10 could resist SNARE zippering at a lower external force than state 9, state 10 must have higher mechanical stability than state 9. The comparison suggests that Munc18-1 associated with the SNARE complex differently in the presence and absence of the NRD. Therefore, the NRD regulates Munc18-1’s interaction with the SNARE bundle and is required to stabilize the SNARE complex in the half-zippered state (Shen et al., 2007; Dulubova et al., 2007).

Munc18-1 induces t-SNARE folding

Next, we pulled the Munc18-bound state 11 to high forces. We saw a small extension jump in a force range of 22-28 pN, showing that the Munc18-bound state 11 unfolded into the NTD-unfolded state 5 (Figure 11A, indicated by magenta arrows). We inferred that state 11 has a conformation similar to the NTD-unfolded state 5, except that Munc18-1 is associated with a structured Tc in a way similar to the Vc peptide (Figure 11E). Indeed, upon SNARE binding Munc18-1 induced approximately equal extension shortening (2.5 ± 0.7 nm) from state 5 as the Vc peptide (2.3 ± 0.5 nm) did. Therefore, in the absence of NRD, Munc18-1 tightly bound t-SNARE and structured Tc. Because SNARE zippering was attenuated, Munc18-1 must also bind amino acids in t-SNARE N-terminal to −1 layer to interfere with NTD zippering (Figure 11E). Accordingly, we estimated that in state 10 VAMP2 was zippered to a position between −2 and −1 layers, in contrast with the half-zippered state 9 (between 0 and +1 layers). These observations suggest that Munc18-1 and the Vc peptide probably promote membrane fusion by the same mechanism: They structure Tc, stabilize the t-SNARE complex, and inhibit SNARE mis-assembly (Pobbati et al., 2006), which outcompete their adverse effects of attenuating SNARE zippering. Finally, we found that Munc18-1 occasionally (4 out of 113) bypassed the NRD to similarly attenuate zippering and structure Tc of the SNARE complex containing the NRD (Figure 11- figure supplement 2,3). This finding suggests that Munc18-1 may transit between the NRD-dependent and the NRD-independent SNARE-binding modes, consistent with previous observations (Rathore et al., 2010; Hu et al., 2011).

In conclusion, we observed that Munc18-1 interacts with the SNARE bundle in at least two modes and differentially regulates SNARE zippering: In an NRD-dependent mode, Munc18-1 stabilizes the half-zippered state, while in an NRD-independent mode, Munc18-1 structures Tc.

Munc18-1 only loosely closes syntaxin

Upon relaxation of the completely unfolded SNARE complex in the presence of Munc18-1, partial refolding of the complex was sometimes observed (17 out of 113 SNARE complexes tested) (Figure 12A). The refolding process was reversible and fast in the force range of 4-8 pN, with an average equilibrium force of 6.1 (±0.8) pN and an extension change of ~4 nm (Figure 12B). This transition required both Munc18-1 and the NRD, because the transition disappeared when either Munc18-1 was omitted or the NRD was removed. We concluded that the transition resulted from the Munc18-1-mediated transition of the syntaxin molecule between the closed conformation and the open conformation (Figure 12C) (Dulubova et al., 1999). The structure of the open conformation was not determined. Consequently, we estimated a lower limit of ~−7 kBT for the free energy of the closed state relative to the open state, based on the measured mechanical work required to unfold the closed state. The relatively small energy difference revealed that the closed syntaxin could spontaneously open to participate in SNARE assembly. This finding is surprising, because it is generally believed that Munc18-1 tightly binds the closed syntaxin with nano-molar affinity, or −20 kBT association free energy (Burkhardt et al., 2008; Misura et al., 2000; Colbert et al., 2013). However, our measurement is consistent with a recent observation that syntaxin can spontaneously open (Hu et al., 2011; Pertsinidis et al., 2013). Given the overall low frequency to observe the syntaxin transition under our experimental conditions (<0.01 s-1), Munc18-1 must remain attached to the syntaxin molecule during the whole syntaxin transition process (Figure 12B), suggesting a multivalent interaction between Munc18-1 and syntaxin (Colbert et al., 2013; Hu et al., 2011; Burkhardt et al., 2008). This finding shows that Munc18-1 binding and syntaxin closing do not necessarily coincide: syntaxin could stay in an open state while Munc18-1 remained attached to part of the syntaxin molecule, including the NRD (Figure 12C) (Hu et al., 2011). The multivalent interaction also reconciles the marginal stability of the closed syntaxin observed by us and the overall high affinity between Munc18-1 and syntaxin.

Figure 12. Munc18-1 only loosely closes syntaxin.

Figure 12.

(A) FECs obtained by pulling (black) and then relaxing (cyan) the SNARE complex. A magenta oval marks the Munc18-1-mediated syntaxin opening and closing transition illustrated in C. A black arrow indicates the t-SNARE unfolding event. (B) Time-dependent extension (black) and force (blue) showing opening and closing transitions of syntaxin as the SNARE complex was being relaxed in the presence of 10 µM Munc18-1. (C) Diagram of the derived syntaxin conformational transition.

DOI: http://dx.doi.org/10.7554/eLife.09580.030

To confirm the above observation, we pulled a single cytoplasmic syntaxin molecule from its C-terminus and a cysteine residue inserted after amino acid D25 following the N-peptide (Figure 13A,B). The N-peptide was free to bind Munc18-1 (Burkhardt et al., 2008; Rathore et al., 2010). Syntaxin alone unfolded in a force range of 15-25 pN and refolded at 3-7 pN, due to irreversible unfolding and refolding of the Habc domain (Figure 13C). In the presence of 10 µM Munc18-1 in the solution, we found another transition in the force range of 3-8 pN that only occurred in the presence of the folded Habc, which represents the Munc18-1-mediated syntaxin opening and closing transition (Figure 13B). The transition was reversible (FECs #4 and #2), but with much smaller transition rate than that seen in the previous construct (Figure 12B). As a result, the extension flicking during pulling or relaxation was not seen in some FECs, such as FEC #3 in Figure 13C. Thus, the syntaxin transition took place in a similar low-force range with a similar extension change as observed in the previous SNARE construct (Figure 12C), confirming the marginal stability of the closed syntaxin state. As a result, the presence of NRD did not significantly reduce the probability for Munc18-1 to mediate de novo SNARE assembly (Figure 9B), although the unfolded SNARE motif in syntaxin could alternatively enter the closed state (Figure 12C). The different transition kinetics seen in the two syntaxin constructs is not surprising, because the syntaxin molecule was pulled in approximately perpendicular directions (compare Figure 13A to Figure 12C). It is known that protein folding kinetics, but not folding energy, strongly depends on the pulling direction (Gao et al., 2011).

Figure 13. Opening the closed syntaxin by force.

Figure 13.

(A) Syntaxin construct pulled from its N- and C-termini to study the syntaxin conformational transition mediated by Munc18-1 (not shown). The syntaxin molecule contained a C-terminal Avi-tag and a cysteine inserted after amino acid D25, which was used to crosslink syntaxin to the DNA handle. (B) Predicted conformational transitions of the syntaxin molecule induced by force. (C) Representative FECs in the absence (−) and presence (+) of Munc18-1 confirming the predicted conformational transitions shown in (B). FECs, force-extension curves.

DOI: http://dx.doi.org/10.7554/eLife.09580.031

Energetics and kinetics of SNARE assembly underlying exocytosis

Our above measurements provide a basis to understand SNARE-mediated membrane fusion. We found that SNARE assembly exhibited different sensitivity to mutations that correlates with their various phenotypes in vivo. Compared to the wild-type SNARE complex, the NTD mutation V39A/V42A reduces the number of docked vesicles, but does not change the Ca2+-triggered fusion rate of the vesicles in the readily releasable pool in chromaffin cells, as was derived from electrophysiological measurements (Walter et al., 2010). In parallel, our measurements showed that the same mutation destabilized NTD by 3 kBT with no change in CTD zippering energy (Figure 7). The comparison suggests that NTD association is responsible for docking, but not vesicle fusion and that the NTD folding energy dictates the number of docked vesicles. Accordingly, the NTD association and dissociation reaches dynamic equilibrium, consistent with dynamic vesicle docking and undocking observed in vivo and in vitro (Zenisek et al., 2000; Zhang et al., 2015). Thus, we predicted that the reduced NTD association rate of the mutant observed by us (Figure 5A) should decrease the fusion rate of the vesicles in the sustained releasable pool (SRP). Indeed, the SRP fusion rate of the mutant is reduced by ~50% (Walter et al., 2010), confirming the prediction. Therefore, NTD association energy and kinetics contribute to the magnitude and rate of vesicle docking, respectively.

Mutations that decreased CTD zippering energy by ~10 kBT, including L70A (+4) and F77A (+6) in VAMP2 and M71A/I192A (+5) in SNAP-25B, also dramatically reduce the rate of exocytosis (Walter et al., 2010; Mohrmann et al., 2010). Interestingly, I67N (+4) in SNAP-25B is a dominant mutation identified from a patient with myasthenia, ataxia, and intellectual disability (Shen et al., 2014). It is found that this mutation impaired neuromuscular transmission. These results demonstrated that the layers +4, +5, and +6 are crucial for CTD zippering and membrane fusion. In contrast, syntaxin T251I (+7) in syntaxin enhanced CTD zippering and is found to increase both spontaneous and evoked exocytosis (Lagow et al., 2007). However, flies carrying this mutation become paralyzed at 38°C. These findings are consistent with the existence of a metastable partially zippered SNARE complex in the docked state (Gao et al., 2012; Kyoung et al., 2011; Lou et al., 2015; Shin et al., 2014) and mutations that stabilize CTD destabilize the half-zippered SNARE complex, leading to mis-regulated exocytosis and reduced precision of neurotransmission. Thus, the stabilities of different SNARE domains appear to be optimized to balance the accuracy and speed of membrane fusion. Finally, other CTD mutations, A67S (+3) and L84A (+8), do not significantly change the CTD folding energy and rate, nor exocytosis (Walter et al., 2010). In conclusion, CTD zippering directly drives membrane fusion by tightly coupling its folding energy to lowering the energy barrier of membrane fusion, thereby increasing the fusion rate.

R56A reduced SNARE zippering energy (Figure 7) and was found to impair membrane fusion in some reports (Ossig et al., 2000). Other MD mutations L60A (+1) and L63A (+2) abolished the independent MD transition and thus changed the SNARE folding pathway. Yu et al. recently examined the impact of both mutations in synaptic exocytosis using cultured mouse neurons (Yu et al., 2015). They found that the two mutations abolished both spontaneous and evoked exocytosis, implying an important role of independent MD assembly in exocytosis. The comparison suggests that an obligate pathway of SNARE assembly may be required for membrane fusion.

Discussion

Synaptic SNARE assembly underlies the strength, speed, and precision of neurotransmission, as well as many neurological disorders. Because SNAREs assemble in multiple stages, SNARE folding intermediates, energetics, and kinetics are intrinsically coupled, making it difficult to characterize SNARE assembly using traditional experimental approaches. By applying high-resolution optical tweezers, we have systematically measured the folding energies and kinetics of both wild-type and mutant SNARE complexes in the absence and presence of Munc18-1. Because of the stage-wise SNARE assembly, crosslinking at the N-terminal edge of NTD (Figure 1B) slightly affects the measured NTD energy, but not energies and kinetics of other domains (Gao et al., 2012; Zorman et al., 2014). In addition, the NTD energies of the mutants relative to that of the WT barely change with the crosslinking site. Combining our findings with previous results on exocytosis, we confirmed distinct functions of different SNARE assembly stages in synaptic exocytosis.

We showed that tight thermodynamic coupling requires specific SNARE assembly intermediates and pathways. MD mutations cause significant heterogeneity in SNARE assembly kinetics and/or abolish independent MD assembly. Furthermore, the MD is targeted by many regulatory proteins that control SNARE assembly, including complexin (Chen et al., 2002; Sudhof and Rothman, 2009; Krishnakumar et al., 2011) and synaptotagmin (Choi et al., 2010; Zhou et al., 2015; Chapman, 2008). Thus, the SNARE engine consists of four stages of zippering in NTD, MD, CTD, and LD with distinct functions. The NTD is responsible for initiating specific formation of the trans-SNARE complex and docking vesicles to the plasma membrane (Walter et al., 2010). The MD serves as a checkpoint to further ensure proper SNARE assembly and as a master switch to control CTD assembly. The CTD acts as a power stroke that directly drives membrane fusion. Continued zippering to LD and the transmembrane domains may provide additional energy for membrane fusion (Stein et al., 2009) or alter the interactions between SNAREs and membranes to facilitate fusion (Ngatchou et al., 2010; Liang et al., 2013; Honigmann et al., 2013).

We found that Munc18-1 regulates every stage of SNARE assembly. Combining with previous results, we propose a working model to account for the multiple roles of Munc18-1 in stage-wise SNARE zippering and membrane fusion (Figure 14). First, we confirmed the previous observation that Munc18-1 only loosely closes syntaxin and associates with open syntaxin (states i and ii) (Hu et al., 2011; Christie et al., 2012). The marginal stability of the closed syntaxin may explain why Munc13 further enhances syntaxin opening, despite the weak interaction between Munc13 and syntaxin (Ma et al., 2013; Ma et al., 2011). Second, we observed that Munc18-1 efficiently initiates SNARE assembly (from state ii to state v). Because this activity is NRD-independent, Munc18-1 likely directly binds SNARE motifs to promote SNARE assembly (states ii and iii) (Shi et al., 2011). Third, Munc18-1 stabilizes the half-zippered SNARE complex in an NRD-dependent manner (state v). This activity is strongly force-dependent and disappears at a force below ~15 pN. Fourth, we found that Munc18-1 associates with the t-SNARE complex (Zhang et al., 2015; Pertsinidis et al., 2013) and induces Tc folding in an NRD-independent manner (state vi). Finally, we did not find evidence that Munc18-1 stabilized the fully assembly SNARE complex in our single-molecule experiments, consistent with a recent report (Zhang et al., 2015). Although Munc18-1 is shown to stabilize trans-SNARE complexes in another report, the effect of stabilization is only minor (Lou et al., 2015). Thus, we conclude that Munc18-1 mainly enhances membrane fusion by catalyzing SNARE assembly, rather than by stabilizing the fully assembled SNARE complex. Consistent with this view, the rate of membrane fusion poorly correlate with the binding affinity between SM proteins and the fully assembled SNARE complexes (Shen et al., 2007; Shen et al., 2015). In particular, SNARE mutations that compromise interactions between the fully assembled SNARE complexes and their cognate SM proteins can support membrane fusion (Peng and Gallwitz, 2004). Taking together, we conclude that Munc18-1 mainly acts on the folding intermediates of SNAREs to chaperone their assembly.

Figure 14. Working model of Munc18-1-regulated stage-wise SNARE assembly in membrane fusion.

Figure 14.

See the main text for details. Munc18-1 undergoes a conformation transition to open the syntaxin molecule (from states i to ii) and form the VAMP2 binding surface (Hu et al., 2011; Parisotto et al., 2014). Thus, syntaxin opening and the template formation in state iii may be cooperative, which likely leads to a transient open syntaxin conformation shown in state ii.

DOI: http://dx.doi.org/10.7554/eLife.09580.032

The Munc18-1-regulated SNARE assembly observed by us corroborates or clarifies many key findings on the role of SM proteins in SNARE assembly and membrane fusion. During revision of this work, Baker et al. reported the crystal structures of fungus SM protein Vps33 bound with its cognate individual Vam3 and Nyv1 SNAREs (Baker et al., 2015). These proteins mediate vesicle fusion with vacuoles or endosomes. In particular, Vam3 and Nyv1 are homologs of syntaxin and VAMP2 belonging to the same Qa- and R-SNARE families (Fasshauer et al., 1998), respectively. They found that Vps33 interacts with the entire Qa- and R-SNARE motifs through two non-overlapping surfaces on Vps33 and aligns the SNARE helical NTDs in proximity and register (state iii). Because the structures of all SNARE complexes and SM proteins are highly conserved, they predicted that SM proteins serve as a template to initiate SNARE assembly into a partially zippered complex. Our discoveries of Munc18-1-mediated de novo SNARE assembly and half-zippered SNARE complex strongly support this prediction, which in turn offers a molecular mechanism for our observations (state iii). In addition, we previously showed that representative SNARE complexes mediating diverse membrane trafficking pathways slowly initiate their NTD assembly and pause in half-zippered states. These observations make SM-mediated SNARE assembly necessary. Our findings also corroborates that Munc18-1 enhances assembly of trans-SNARE complexes, thereby promoting liposome-liposome fusion (Rathore et al., 2010; Shen et al., 2007; Shen et al., 2015). Finally, the N-peptide is essential for recruiting Munc18-1 to the fusion site to assist SNARE assembly (Rathore et al., 2010). Interestingly, once the trans-SNARE complexes are formed, the N-peptide is not required and can be cleaved from syntaxin SNARE motif without compromising the subsequent liposome fusion in vitro, indicating that Munc18-1 binds the trans-SNARE complex in an NRD-independent manner before fusion (state vi). Consistent with this observation, we considered that after trans-SNARE assembly, Munc18-1 switches to the NRD-independent Tc binding mode observed by us. Munc18-1 then induces Tc folding and greatly stabilizes the t-SNARE to facilitate SNARE assembly and membrane fusion similar to Vc and Vn peptides (Melia et al., 2002; Pobbati et al., 2006; Li et al., 2014). Moreover, our results are consistent with other potentially essential roles of SM proteins in membrane fusion, which are to protect disassembly of t- and trans-SNARE complexes by NSF (Xu et al., 2010a; Lobingier et al., 2014; Zhao et al., 2015) and to proofread SNARE zippering (Lobingier et al., 2014). These comparisons suggest that SM proteins act as chaperones to enhance SNARE assembly, which is essential for membrane fusion.

Our findings contrast with previous reports that Munc18-1 reduces the rate of SNARE assembly in an NRD-dependent manner, probably due to different experimental conditions (Burkhardt et al., 2008). We noticed that Munc18-1 and other SM proteins significantly enhance membrane fusion only under special conditions. Shen and co-workers showed that incubating SNARE-anchored liposomes in the presence of Munc18-1 at 4ºC or adding crowding agents, such as 100 mg/ml Ficoll 70, in the fusion reaction is required to observe Munc18-1-enhanced liposome fusion (Shen et al., 2007; Yu et al., 2015). In general, SM proteins appear to weakly associate with both Qa- and R-SNAREs to form the template that initiates SNARE assembly (Parisotto et al., 2014; Xu et al., 2010b; Baker et al., 2015; Lobingier and Merz, 2012). The energy barrier for syntaxin to transit from a closed conformation to an open conformation further impedes formation of the template between Munc18-1 and syntaxin (Hu et al., 2011; Baker et al., 2015). The use of N-terminally crosslinked SNARE constructs in our experiments may facilitate Munc18-1 binding to both syntaxin and VAMP2 to form the template required for SNARE assembly (state iii). In addition, the presence of a single SNAP-25 molecule in our experiments may increase the contrast to observe Munc18-1-mediated de novo SNARE assembly. With a high concentration of SNAP-25 in the solution in ensemble experiments, the SM-mediated SNARE assembly may be obscured by the high rate of intrinsic SNARE assembly (Baker et al., 2015).

Evidence suggests that Munc18-1 greatly accelerates assembly of the SNAREs on the liposomes that are already docked (Shen et al., 2007; Yu et al., 2015). Munc18-1 may orchestrate a specific number of trans-SNARE complexes (state vii) (Mohrmann et al., 2010; Karatekin et al., 2010; Megighian et al., 2013; Hernandez et al., 2014; Lu et al., 2008) to cooperatively zipper. Our measurements showed that most of the mutant SNARE complexes are still more stable than many SNARE complexes mediating other membrane trafficking pathways (Zorman et al., 2014). As a result, SNARE-mediated fusion in the absence of Munc18-1 is remarkably insensitive to CTD folding energies (Zorman et al., 2014; Shen et al., 2007). We hypothesize that Munc18-1 helps to form a super-complex containing Munc18-1, trans-SNARE complexes, and other regulatory proteins with approximately fixed stoichiometry to efficiently and specifically drive membrane fusion. Without Munc18-1-dependent constraints on the number of trans-SNARE complexes, the energy loss caused by SNARE mutation may be compensated by the energy gain from recruitment of more SNARE complexes to the fusion site. As a result, membrane fusion mediated by SNARE alone has variable number of SNARE complexes involved (Hernandez et al., 2014), which causes non-specific membrane fusion. Thus, Munc18-1 intimately chaperone SNARE folding from syntaxin to multiple trans-SNARE complexes, making it indispensable for SNARE-mediated membrane fusion.

Materials and methods

Protein purification, labeling, and SNARE complex formation

All recombinant proteins were expressed in BL21 E. coli cells and purified using His-tags. Syntaxin was biotinylated at the Avi-tag in vitro using the biotin ligase (Gao et al., 2012). The His-tag was removed from purified syntaxin and VAMP2, but kept in other proteins. SNARE complexes were formed overnight by mixing syntaxin and VAMP2 in 1:1 molar ratio and an excessive amount of SNAP-25B and then purified using the His-tag on SNAP-25.

Dual-trap optical tweezers

The dual-trap optical tweezers were home-built and calibrated as previously described (Gao et al., 2012; Sirinakis et al., 2012; Moffitt et al., 2006). Briefly, a laser beam with a wavelength of 1064 nm was expanded, collimated, and split into two orthogonally polarized beams. One beam was reflected by a mirror attached to a nano-positioning stage that could tip/tilt in two axes with high resolution (Mad City Labs, WI). The two beams were then combined, further expanded, and focused by a water-immersion 60X objective with a numerical aperture of 1.2 (Olympus, PA) to form two optical traps. One optical trap was moved by turning the mirror to control the force applied to a single molecule. The outgoing laser beams were collimated by an identical objective, split again by polarization, and projected to two position-sensitive detectors (Pacific Silicon Sensor, CA) to detect bead positions using back-focal-plane interferometry. The force constants of both optical traps were calibrated by Brownian motion of the trapped beads (Zhang et al., 2012). The force, extension, trap separation, and other experimental parameters were acquired at 20 kHz, filtered online to 10 kHz, and stored on hard-disk.

Single-molecule experiments

The SNARE complex was mixed with the DNA handle at a molar ratio of 50:1 and crosslinked by exposing the solution to air overnight to oxidize the thiol groups (Gao et al., 2012). An aliquot of the mixture was bound to anti-digoxigenin antibody-coated polystyrene beads. A single such bead was subsequently captured in one optical trap and brought close to a streptavidin-coated bead in a second trap to form the protein-DNA tether between the two beads. All SNARE pulling experiments were carried out in phosphate-buffered saline supplemented with an oxygen-scavenging system at room temperature.

Data analysis

The data analysis yielding the intermediates and energies was performed as previously described (Gao et al., 2012) and detailed in a manuscript using the SNARE complex containing the VAMP2 R56A mutant as an example (Rebane, et al., 2016). We normally performed the HMM analysis for the whole extension-time trajectory obtained at each trap separation that typically lasted 5–300 s, after the trajectory was mean-filtered to 5 kHz or 1 kHz. We calculated the histogram distribution of the extension and determined the number of states by fitting the distribution with multiple Gaussian functions. Then, we optimized the parameters in the hidden Markov model using gradient descent (Qin et al., 2000). Finally, the idealized extension trajectories were calculated using the Viterbi algorithm (Rabiner, 1989).

We chose the contour length of the unfolded and stretched polypeptide l as a reaction coordinate to describe SNARE folding along a pathway inferred from the crystal structure of the fully assembled SNARE complex (Sutton et al., 1998; Stein et al., 2009). We first derived the conformation of the t-SNARE complex in state 5 based on its extension relative to the fully unfolded state 6 (Gao et al., 2012) (Figure 1D) and the Vc-bound state 8 (Figure 3). The derived t-SNARE conformation is also supported by our experiments directly pulling a single t-SNARE complex from the C-termini of syntaxin and SNAP-25 (unpublished results). We assumed that NTD and MD zippering proceeded by folding of VAMP2 on the structured t-SNARE template and that CTD zippering was accompanied by concurrent folding of both VAMP2 and Tc. The LD transition was considered to be symmetrical zippering of syntaxin and VAMP2 and was characterized as before (Gao et al., 2012). To derive conformations of the intermediate and transition states in the folding pathway from the overlapping CTD, MD, and NTD transitions, we defined a simplified energy landscape (li,Vi), characterized by the contour length lof i-th intermediate state or transition state and its associated free energy Vi at zero force. These parameters were determined by fitting the model-based calculations to the experimental measurements. To do so, we first established the experimental observables as a function of the simplified energy landscape. We calculated the total extension Xi and energy Gi for each state in the presence force. Both quantities constituted contributions from three components: the unfolded polypeptide, the folded portion of the protein, and the DNA handle (Figure 2—figure supplement 3). The total energy additionally contained the potential energy of two beads in optical traps. Thus, the extension of the protein-DNA tether was calculated as

Xi = xi(m) + Hi + xi(DNA) (1)

Here, the force-dependent extension of the unfolded polypeptide or the DNA handle is described by the Marko-Siggia formula for a semi-flexible worm-like chain (Marko and Siggia, 1995), i.e.,

Fi=kBTP14(1xiL)2+xiL14, (2)

where Fis the average force of state i and P and L are the persistence length and the contour length of the chain, respectively. We chose = 40 nm and L = 768.4 nm for DNA (Bustamante et al., 1994) and P = 0.6 nm and L = li for the polypeptide (Gao et al., 2011; Xi et al., 2012). The extension of the folded protein portion was calculated based on a freely jointed chain model (Smith et al., 1992)

Hi=-kBTFi+hi cothFihikBT, (3)

where his the size the folded protein portion in state i along the pulling direction, which was measured from the crystal structure as a function of the contour length l of the unfolded polypeptide. The tether extension is related to the experimental control parameter trap separation D by the following formula

D=Xi+Fiktraps+R, (4)

where Fi/ktraps is the total bead displacement with ktraps = k1k2/(k1+k2) the effective trap stiffness of the two optical traps and R the sum of the bead radii. Given the experimental conditions and contour length of a state li, we could solve its state force Fi by substituting Equations 1–3 into Equation 4. Similarly, we could calculate the total energy of the system as

Gi=Gim+Vi+Gi(DNA)+Fi22ktraps, (5)

where Gi(m), Gi(DNA), and Fi2/(2ktraps) are the energies of the unfolded polypeptide, the DNA handle, and the beads in optical traps, respectively. The former two energies result from entropy changes of the worm-like chains due to stretching, which were calculated as

Gi(m or DNA)=kBTPL41-xiL3xiL2-2xiL3. (6)

Given the state energies, we computed the state populations based on the Boltzmann distribution and the transition rates in terms of Kramers’ formula. Finally, we simultaneously fit the calculated state forces, populations, transition rates, and extension changes to the corresponding measurements using the nonlinear least-squares method, yielding the best-fit parameters for the simplified energy landscape.

Acknowledgements

We thank James Rothman, Frederick Hughson, Thomas Söllner, Jingshi Shen, Erdem Karatekin, Shyam Krishnakumar, Frederic Pincet, Xinming Zhang, and Junyi Jiao for discussion and reading the manuscript, Hong Qu, Bowei Su, and Haijia Yu for help in experiments, and Mengze He for preparing the videos. This work was supported by the NIH grant RO1GM093341 to Y. Z. Research reported in this publication was also supported in part by the Brain Research Foundation and by the Raymond and Beverly Sackler Institute for Biological, Physical and Engineering Sciences at Yale.

Funding Statement

The funders had no role in study design, data collection and interpretation, or the decision to submit the work for publication.

Funding Information

This paper was supported by the following grants:

  • National Institutes of Health GM093341 to Yongli Zhang.

  • Raymond and Beverly Sackler Institute for Biological, Physical and Engineering Sciences, Yale University to Yongli Zhang.

Additional information

Competing interests

The authors declare that no competing interests exist.

Author contributions

LM, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article, Contributed unpublished essential data or reagents.

AAR, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article.

GY, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article, Contributed unpublished essential data or reagents.

ZX, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article.

YK, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article.

YG, Conception and design, Acquisition of data, Analysis and interpretation of data, Drafting or revising the article.

YZ, Mentoring, Conception and design, Analysis and interpretation of data, Drafting or revising the article.

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eLife. 2015 Dec 23;4:e09580. doi: 10.7554/eLife.09580.033

Decision letter

Editor: Stephen C Harrison1

In the interests of transparency, eLife includes the editorial decision letter and accompanying author responses. A lightly edited version of the letter sent to the authors after peer review is shown, indicating the most substantive concerns; minor comments are not usually included.

Thank you for submitting your work entitled "Munc18-1-regulated stage-wise SNARE assembly underlying synaptic exocytosis" for peer review at eLife. Your submission has been favorably evaluated by Vivek Malhotra (Senior Editor), and three reviewers, one of whom is a member of our Board of Reviewing Editors.

The reviewers have discussed the reviews with one another and the Reviewing Editor has drafted this decision to help you prepare a revised submission.

Summary:

This paper describes a technically impressive study, in which the authors used an optical tweezers to map out the energetics and kinetics of neuronal SNARE assembly. Two technical features distinguish this work from earlier efforts. First, the authors figured out how to crosslink VAMP and syntaxin so that they could observe assembly as well as disassembly. Second, they determined assembly energetics/kinetics for a well-chosen set of VAMP (and a small number of syntaxin and SNAP-25) mutants. They then went on to determine assembly energetics/kinetics in the presence of Munc18. The authors demonstrate: (1) that regions within the SNARE bundle are responsible for a series of assembly intermediates (at least under the conditions of the experiment) that they propose correspond to well-characterized stages in vesicle docking and membrane fusion: (2) that Munc18 can bind and influence the structures and energetics of SNARE assembly intermediates, providing support for the idea that Munc18 functions as an assembly chaperone.

Essential revisions:

The paper is, in some respects, two separate reports. In one, the authors characterize 15 different SNARE-complex mutants, previously studied by different methods and in different experimental setting. As the authors correctly point out, a coherent treatment by a uniform method is needed. In the other, the authors examine the effects of Munc18 on assembly and disassembly of single SNARE complexes. There are many new observations and insights, but the conclusions are less convincing than those of the first part (see below).

Major comments:

Overall:

(a) The paper’s structure needs to be reorganized. Some important points are treated summarily (see last paragraph under "part 1", below), while some irrelevant ones are emphasized.

(b) Please take care not to base structural interpretations on single distance measurements. While the models for states 1-8 are undeniably useful, and while the mutagenesis results as well as previous studies provide some additional support, the models should be presented and discussed more cautiously. Even the presence or absence of, for example, SNAP-25 in each of these states does not strike the reviewers as a foregone conclusion.

(c) As a specific example of interpretive ambiguity, the authors assume for the unfolding state 4 in Figure 1D that syntaxin (and probably also, SNAP-25) is partially disassembled up to layer +5. It is also possible, however, that the t-SNARE α-helices remain intact, while unfolding of VAMP2 progresses beyond the point shown, for example, up to layer -1 or -2. How do the authors differentiate between these possibilities? Since the C-terminal fragment of VAMP2 (VAMP2 49-96) induces tight folding of the C-terminal part of the t-SNARE proteins (many data in the previous literature and Figure 5E in this manuscript), addition of the C-terminal VAMP2 fragment should decrease the extension value of states 4 and 5 if the t-SNARE complex is indeed partially melted as the authors suggest. The authors might also (in part 2) repeat this experiment with Munc18, because they claim that Munc18, like the C-terminal VAMP2 fragment, chaperones the C-terminal end of the t-SNARE complex.

(d) The suggested switching of Munc-18 interactions likewise appears to be arbitrary. The authors make no effort to justify that interpretation in terms of what is known about Munc18 structure and biochemistry. There are many ways in which two apparently distinct activities can be interpreted, without requiring distinct modes of interaction. The authors overstate the case by saying (rather pompously) "we discovered (sic) that Munc18-1 interacts with the SNARE bundle in at least two distinct modes".

(e) The authors claim that they have "quantitatively verified the tight thermodynamic coupling between SNARE zippering and membrane fusion and revealed distinct functions of different SNARE assembly stages." They have done nothing of the kind. They have done a fine job of detecting intermediates in a useful and valuable model, in which individual SNARE complexes are pulled and relaxed, and they can (and should) be pleased with that accomplishment. But when several SNARE complexes are pulling on the same two membranes and the membranes are pulling back on them, as is the case for exocytic fusion (indeed, membrane fusion generally), then the relative heights of barriers, etc., might well be different. That difference doesn't diminish the value of the numbers provided here, but it does rule out egregious overstatement. Even the interpretation in the third paragraph, subsection “Energetics and kinetics of SNARE assembly underlying exocytosis”, seems stretched – why do the phenotypes of those mutations reveal "an essential role of independent MD assembly"? Yes, messing up the MD messes up the mouse, but how does even the correspondence to the kinetic observations reported here demonstrate "independent" (rather than "concerted", with the other segments) assembly?

Part 1:

Although the authors basically performed the same experiments as in Gao et al. (2012), there seem to be two differences. The first is that unfolding in the C-terminal half of the SNARE complex, previously treated as one process, has now been resolved into CTD and MD unfolding (states 3 and 4), presumably because they did less temporal averaging of the data and plotted the extension traces over 1kHz. The second difference is that they moved the crosslinking site to layer -6. This difference likely separated NTD unfolding (state 5) from dissociation of SNAP-25 (state 6) more clearly than in Gao et al. (2012), in which the crosslinker was at layer -7. Thus, before dissociation of SNAP-25 at a higher force, they could see reversible NTD unfolding and refolding transitions.

In Figures 2 and 3, the authors used the high temporal (over 1 kHz) and spatial resolution provided by the optical tweezers to resolve detailed structural transitions occurring in a single neuronal SNARE complex – a substantial technical accomplishment. They resolve the C-terminal unfolding into two intermediates (3 and 4). The transition between the two involves unfolding (or refolding) of the middle part between the +2 and the zeroth layers (but this analysis may need to be refined). The mutations in the +1 or +2 layer accordingly affect the stability of these intermediates. Thus, the probability of observing intermediate 3 is selectively reduced (i.e., the unfolding process pauses less frequently at the +2 layer).

The authors claim that "the middle domain plays a pivotal role in robust and correct stage-wise SNARE assembly, and its mutation leads to changes in SNARE assembly pathway and accuracy" and that "the MD serves as a checkpoint to further ensure proper SNARE assembly as a master switch to control CTD assembly". It is hard to understand how the reduced observation of the intermediate 3 (observed for the L60A and L63A mutants) supports these rather strong arguments. In the third paragraph of the subsection “Energetics and kinetics of SNARE assembly underlying exocytosis”, the authors allude to unpublished results, but this citation is not an appropriate way to justify the arguments. The authors should either weaken these claims or provide experimental evidence to support their arguments.

Part 2:

Data showing different effects of Munc18 are mixed confusingly together, making part 2 extremely hard to follow, even for a reader who knows the field. In particular, in Figure 5 and 6, rearrangements of the figure subpanels would improve readability. For example, the subpanels, Figure 5A-C and Figure 6A report that Munc18 helps reassembly of the SNARE complex after complete unfolding of the t-SNARE pre-complexes, so that these panels can be grouped together to make one figure. On the other hand, the subpanels including Figure 5D to G and Figure 6B to D report stabilization of the half-zipped SNARE complex by Munc18, which may be grouped together to make another figure.

From the extension difference between states 8 and 5 (Figure 6B), observed only in the absence of NRD (N-terminal Regulatory Domains), the authors argue that Munc18 would bind to the C-terminal part of the t-SNARE proteins and induce a coil-to-helix transition. But then, state 4 with bound Munc18 should have a smaller extension than state 4 without Munc18.

Figure 7 and the accompanying discussion are not very clear, and the reviewers found the conclusions unconvincing. For example, the opening and closing of syntaxin induced by Munc 18 (Figure 7A and B) is intriguing, but then why do authors not observe reversible transitions between open and closed syntaxin in the more direct pulling study shown in Figure 7C?

Overall recommendation:

1) Present the structural models for the kinetic states more cautiously and explain any alternatives.

2) Support the interpretation of the role of the MD with data (and pay attention to other comments under "part 1", above).

3) When revising what we have called "part 2", comply with each of the three paragraphs under "part 2", above.

4) Provide details (in the Methods) for the nonlinear least-square fitting that converts dwell times to deltaG (or deltaG double dagger).

[Editors' note: further revisions were requested prior to acceptance, as described below.]

Thank you for submitting your work entitled "Munc18-1-regulated stage-wise SNARE assembly underlying synaptic exocytosis" for consideration by eLife. Your article has been reviewed by two peer reviewers, and the evaluation has been overseen by a Reviewing Editor and Vivek Malhotra as the Senior Editor.

The reviewers have discussed the reviews with one another and the Reviewing Editor has drafted this decision to help you prepare a revised submission.

Summary:

The reviewers agreed that the manuscript is greatly improved, but it remains, despite the revision, challenging and complex. In particular, two parts need attention, as follows.

Essential revisions:

A) The subsection entitled "Position-dependent effects of layer mutation on SNARE assembly", in which the authors discuss single-molecule mechanics of 15 SNARE complex mutants, was very difficult to follow. We propose the following changes:

1) In Figure 4, show explicitly the name of the domain (NTD, MTD and CTD) to which each mutant belongs.

2) In the same figure, the current way in which FECs are marked is difficult to recognize. The colors and patterns are too similar. One way is to depict the corresponding transitions right next to individual FEC regions.

3) How is "MD+NTD" different from "MD_NTD"? The reviewers could not find proper explanations neither in the main text nor figure legends.

4) In Figure 5, each mutant trace is labeled with jargon, such as, "M46A CTD+MD_NTD". This labeling is nearly impossible to understand. It may be enough to depict the corresponding domains above the subpanel of Figure 5B (i.e., LC, CTD, MD and NTD). And the readers can then interpret the data as they are.

b) Figure 11 is also hard to follow. The authors introduced new States 10 and 11. Observation of the State 11 was attributed to folding of the C-terminal end of the t-SNARE proteins (called Tc in the manuscript) induced by Munc18-1 binding. An immediate question is whether such Tc structuring was observed in the presence of NRD. Also, the authors argued that the two partially-zipped states, State 9 and State 10, are different from each other (subsection “Munc18-1 induces t-SNARE folding”), which the reviewers could not understand. Because the NRD-truncated SNARE complex has less biological relevance, the authors may want consider moving Figure 11 to supplementary data. The data in Figures 9, 10, 12 and 13 collectively make a smooth flow, but the data in Figure 11 seem at odds with those in the other figures.

eLife. 2015 Dec 23;4:e09580. doi: 10.7554/eLife.09580.034

Author response


Essential revisions:

The paper is, in some respects, two separate reports. In one, the authors characterize 15 different SNARE-complex mutants, previously studied by different methods and in different experimental setting. As the authors correctly point out, a coherent treatment by a uniform method is needed. In the other, the authors examine the effects of Munc18 on assembly and disassembly of single SNARE complexes. There are many new observations and insights, but the conclusions are less convincing than those of the first part (see below). Major comments: Overall: (a) The paper’s structure needs to be reorganized. Some important points are treated summarily (see last paragraph under "part 1", below), while some irrelevant ones are emphasized.

We agree with the comments made by the reviewers. Following the reviewers’ suggestion, we have made a major revision of our manuscript.

(b) Please take care not to base structural interpretations on single distance measurements. While the models for states 1-8 are undeniably useful, and while the mutagenesis results as well as previous studies provide some additional support, the models should be presented and discussed more cautiously. Even the presence or absence of, for example, SNAP-25 in each of these states does not strike the reviewers as a foregone conclusion.

We understand the reviewers’ concern here. The wide applications of optical tweezers in protein folding studies and our research experience in this field have led our belief that optical tweezers can be used to reliably determine the conformations and energies of protein folding intermediates. We have written a separate manuscript dedicated to our methods of data analysis, which was favorably reviewed in another journal. Basically, we combine our high-resolution single-molecule measurements, the crystal structure of the fully assembled SNARE complex, including its linear topology, and results of SNARE mutations, truncations, and protein binding to model the conformations of SNARE intermediates. We have described salient features of our methods, including key mathematical formulae, in the Data Analysis part of the Materials and methods section. In addition, we have added Figure 2—figure supplement 3 to describe how the extension and energy are calculated in our model. Furthermore, we have made three major changes to address the reviewers’ concern:

First, we have moved our description on SNAP-25 binding earlier in the text (subsection “Four stages of SNARE assembly in four domains”).

Second, we have elaborated our method of data analysis in the subsection “Energetics and kinetics of SNARE assembly”.

Finally, we have added a new section “Vc peptide induces folding of t-SNARE C-terminus and attenuates SNARE zippering” to describe effects of Vc peptide on SNARE assembly. As a result, we have added a new main figure, Figure 3. Results from the Vc peptide binding experiment confirmed our structural models shown in Figure 1D.

In conclusion, these revisions, our previous results (Gao et al., 2012; Zorman et al., 2014), and results obtained from complementary approaches obtained in other groups (e.g., Li et al., 2014; Diao et al., 2012), corroborate the data analysis methods and the structural models derived by us.

(c) As a specific example of interpretive ambiguity, the authors assume for the unfolding state 4 in Figure 1D that syntaxin (and probably also, SNAP-25) is partially disassembled up to layer +5. It is also possible, however, that the t-SNARE α-helices remain intact, while unfolding of VAMP2 progresses beyond the point shown, for example, up to layer -1 or -2. How do the authors differentiate between these possibilities? Since the C-terminal fragment of VAMP2 (VAMP2 49-96) induces tight folding of the C-terminal part of the t-SNARE proteins (many data in the previous literature and Figure 5E in this manuscript), addition of the C-terminal VAMP2 fragment should decrease the extension value of states 4 and 5 if the t-SNARE complex is indeed partially melted as the authors suggest. The authors might also (in part 2) repeat this experiment with Munc18, because they claim that Munc18, like the C-terminal VAMP2 fragment, chaperones the C-terminal end of the t-SNARE complex.

The reviewers pointed out an important feature in our data analysis. In our model, SNAREs fold and unfold in a sequential and stepwise manner, between the well-defined fully assembled state (state 1) and the fully unfolded state (state 6). The total extension change is fixed by the extension difference between the two states. We essentially performed an interpolation to locate the conformations of intermediate states based on their measured relative extensions. Thus, an increase in the extension change of one folding step must be compensated by a decrease in the extension change of another folding step. In our analysis, we first determine the t-SNARE conformation (state 5) based on its extension relative to the completely unfolded state (state 6) and the Vc-peptide-bound state (state 8 in Figure 3). The t-SNARE transitions into both states are modeled as helix-coil transitions and the measured extension changes determine the lengths of the syntaxin helix involved in the transitions (please see Fig. S10 in Gao et al., 2012. This analysis reveals a frayed t-SNARE conformation as shown in Figure 1D. This conformation is also supported by our extensive unpublished data on directly pulling the t-SNARE complex. As is hypothesized by the reviewer, we did observe extension shortening due to binding of the Vc peptide 49-96 (Figure 3) and Munc18-1 (Figure 11). Then we simultaneously fit the extensions of the intermediates 2-4 to the experimental measurements to determine the borders of these states. The fitting avoids the scenario proposed by the reviewer, because shifting the border between states 4 and 5 towards the N-terminus will shorten the extension change of NTD transition.

To address the reviewers’ comments, we have made the following changes:

1. Described our method of data analysis in the Materials and methods;

2. Added a new section, Vc peptide induces folding of t-SNARE C-terminus and attenuates SNARE zippering”, to describe effects of Vc peptide on SNARE assembly. As a result, we have added a new main figure, Figure 3. Results from the Vc peptide binding experiment confirmed our structural models shown in Figure 1D.

3. Added Figure 11 to specifically describe NRD-independent binding of Munc18-1 to the t-SNARE C-terminus (Tc).

(d) The suggested switching of Munc-18 interactions likewise appears to be arbitrary. The authors make no effort to justify that interpretation in terms of what is known about Munc18 structure and biochemistry. There are many ways in which two apparently distinct activities can be interpreted, without requiring distinct modes of interaction. The authors overstate the case by saying (rather pompously) "we discovered (sic) that Munc18-1 interacts with the SNARE bundle in at least two distinct modes".

We thank reviewers for the insightful suggestion. Following the suggestion, we have tried to integrate our observations to previous findings on Munc18-1 and also compared the differences in the Discussion part. As a result, we have made major revision in the Discussion part and also the model figure (Figure 14). In particular, we found that our independent observations on Munc18-1-mediated SNARE assembly and half-zippered SNARE complex are in excellent agreement with findings recently reported by Hughson and coworkers (Baker et al., 2015). Finally, we have revised the sentence mentioned by reviewers as follows:

“In conclusion, we observed that Munc18-1 interacts with the SNARE bundle in at least two modes and differentially regulates SNARE zippering: In an NRD-dependent mode, Munc18-1 stabilizes the half-zippered state, while in an NRD-independent mode, Munc18-1 structures Tc.”

(e) The authors claim that they have "quantitatively verified the tight thermodynamic coupling between SNARE zippering and membrane fusion and revealed distinct functions of different SNARE assembly stages." They have done nothing of the kind. They have done a fine job of detecting intermediates in a useful and valuable model, in which individual SNARE complexes are pulled and relaxed, and they can (and should) be pleased with that accomplishment. But when several SNARE complexes are pulling on the same two membranes and the membranes are pulling back on them, as is the case for exocytic fusion (indeed, membrane fusion generally), then the relative heights of barriers, etc., might well be different. That difference doesn't diminish the value of the numbers provided here, but it does rule out egregious overstatement. Even the interpretation in the third paragraph, subsection “Energetics and kinetics of SNARE assembly underlying exocytosis”, seems stretched – why do the phenotypes of those mutations reveal "an essential role of independent MD assembly"? Yes, messing up the MD messes up the mouse, but how does even the correspondence to the kinetic observations reported here demonstrate "independent" (rather than "concerted", with the other segments) assembly?

We are sorry for our overstatements. Fully accepting the reviewers' criticisms, we have revised the relevant sentences as “Combining our findings with previous results on exocytosis, we confirmed distinct functions of different SNARE assembly stages in synaptic exocytosis.”

“SNAREs couple their exergonic folding to membrane fusion (Sudhof and Rothman, 2009; Rothman, 2014). Such a thermodynamic coupling mechanism predicts that any perturbation in SNARE assembly impacts membrane fusion. Significant progresses have been made to test the prediction in the past two decades (Chen et al., 1999; Walter et al., 2010; Mohrmann et al., 2010). However, a quantitative test requires accurate and comprehensive measurements of both the energies and kinetics of SNARE assembly and the rates of membrane fusion for wild-type and various mutant SNARE complexes.”

and

“Other MD mutations L60A (+1) and L63A (+2) abolished the independent MD transition and thus changed the SNARE folding pathway. Yu et al. recently examined the impact of both mutations in synaptic exocytosis using cultured mouse neurons (Yu et al., 2015). They found that the two mutations abolished both spontaneous and evoked exocytosis, implying an important role of independent MD assembly in exocytosis. The comparison suggests that an obligate pathway of SNARE assembly may be required for membrane fusion.”

In addition, we have added many phrases to emphasize numerous previous reports on electrophysiological measurements of exocytosis. For example, in the Abstract:

“We found that SNARE layer mutations differentially affect SNARE assembly. Comparison of their effects on SNARE assembly and on exocytosis reveals that NTD and CTD are responsible for vesicle docking and fusion, respectively, whereas MD regulates SNARE assembly and fusion.”

Finally, we recognize that multiple SNARE complexes are required for membrane fusion, as is shown in our model figure (Figure 14) and had tried to integrate our single-molecule measurement to membrane fusion in our previous work (Zorman et al., 2014).

Part 1: Although the authors basically performed the same experiments as in Gao et al. (2012), there seem to be two differences. The first is that unfolding in the C-terminal half of the SNARE complex, previously treated as one process, has now been resolved into CTD and MD unfolding (states 3 and 4), presumably because they did less temporal averaging of the data and plotted the extension traces over 1kHz. The second difference is that they moved the crosslinking site to layer -6. This difference likely separated NTD unfolding (state 5) from dissociation of SNAP-25 (state 6) more clearly than in Gao et al. (2012), in which the crosslinker was at layer -7. Thus, before dissociation of SNAP-25 at a higher force, they could see reversible NTD unfolding and refolding transitions. In Figures 2 and 3, the authors used the high temporal (over 1 kHz) and spatial resolution provided by the optical tweezers to resolve detailed structural transitions occurring in a single neuronal SNARE complex – a substantial technical accomplishment. They resolve the C-terminal unfolding into two intermediates (3 and 4). The transition between the two involves unfolding (or refolding) of the middle part between the +2 and the zeroth layers (but this analysis may need to be refined). The mutations in the +1 or +2 layer accordingly affect the stability of these intermediates. Thus, the probability of observing intermediate 3 is selectively reduced (i.e., the unfolding process pauses less frequently at the +2 layer).

We thank the reviewers for correctly summarizing our main findings presented in the manuscript.

The authors claim that "the middle domain plays a pivotal role in robust and correct stage-wise SNARE assembly, and its mutation leads to changes in SNARE assembly pathway and accuracy" and that "the MD serves as a checkpoint to further ensure proper SNARE assembly as a master switch to control CTD assembly". It is hard to understand how the reduced observation of the intermediate 3 (observed for the L60A and L63A mutants) supports these rather strong arguments. In the third paragraph of the subsection “Energetics and kinetics of SNARE assembly underlying exocytosis”, the authors allude to unpublished results, but this citation is not an appropriate way to justify the arguments. The authors should either weaken these claims or provide experimental evidence to support their arguments.

Following the reviewers’ suggestion, we have weakened our claim on the significance of the MD, as is described in our preceding replies. During revision of this manuscript, the unpublished work referred in our previous manuscript has been published (Yu et al., 2015). We have updated the citation. The major and common change caused by L60A and L63A is a combination of both CTD and MD into one transition unit, which demonstrates a change in the SNARE assembly pathway. Therefore, we suggest that a conserved SNARE folding pathway, including an independent MD folding, may be required for membrane fusion.

Part 2: Data showing different effects of Munc18 are mixed confusingly together, making part 2 extremely hard to follow, even for a reader who knows the field. In particular, in Figure 5 and 6, rearrangements of the figure subpanels would improve readability. For example, the subpanels, Figure 5A-C and Figure 6A report that Munc18 helps reassembly of the SNARE complex after complete unfolding of the t-SNARE pre-complexes, so that these panels can be grouped together to make one figure. On the other hand, the subpanels including Figure 5D to G and Figure 6B to D report stabilization of the half-zipped SNARE complex by Munc18, which may be grouped together to make another figure.

We thank the reviewers for pointing out our poor figure organization. Following the reviewers’ suggestion, we have made major efforts to re-organize the figures in the whole revised manuscript. We make sure that each figure focuses on one subject matter. We believe these changes substantially improve the readability of the second part of the manuscript.

From the extension difference between states 8 and 5 (Figure 6B), observed only in the absence of NRD (N-terminal Regulatory Domains), the authors argue that Munc18 would bind to the C-terminal part of the t-SNARE proteins and induce a coil-to-helix transition. But then, state 4 with bound Munc18 should have a smaller extension than state 4 without Munc18.

The reviewers would be right if VAMP2 were free to zipper in this case. However, the average extension change upon NTD zippering on Munc18-1 bound t-SNARE complex (between states 10 and 11 in Figure 11C) is smaller than the corresponding extension change in the absence of Munc18-1 (between states 4 and 5 in Figure 2B). This indicates that VAMP2 can only zipper to a position N-terminal to -1 layer in the presence of bound Munc18-1, which prevents VAMP2 from zippering to a position corresponding to state 4. We designated this new position as state 10 in Figure 11 and illustrated its different position in Figure 11E. Note that due to its short lifetime, state 4 is not always clearly seen in some extension-time trajectories exhibited at 1000 Hz, as is stated in the main text.

Figure 7 and the accompanying discussion are not very clear, and the reviewers found the conclusions unconvincing. For example, the opening and closing of syntaxin induced by Munc 18 (Figure 7A and B) is intriguing, but then why do authors not observe reversible transitions between open and closed syntaxin in the more direct pulling study shown in Figure 7C?

We appreciate that the reviewers pointed out the difference. Closed inspection showed that the transition in this new pulling direction is indeed reversible, as is seen in one of the force-extension curves shown (Figure 13, FEC #2). We have now added a new FEC to better exhibit the reversible transition (FEC #4). The transition rate is much lower than that seen in the previous construct (Figure 12). We have clarified the difference in the main text as follows:

“The transition was reversible (FECs #4 and #2), but with much smaller transition rate than that seen in the previous construct (Figure 12B). As a result, the extension flicking during pulling or relaxation was not seen in some FECs, such FEC #3 in Figure 13B.”

“The different transition kinetics seen in the two syntaxin constructs is not surprising, because the syntaxin molecule was pulled in two approximately perpendicular directions (compare Figure 13A to Figure 12C). It is known that protein folding kinetics, but not folding energy, strongly depends on the pulling direction (Gao et al., 2011).”

Overall recommendation: 1) Present the structural models for the kinetic states more cautiously and explain any alternatives.

Yes, we have done so. Please see our response to the Major comments (b) and (c).

2) Support the interpretation of the role of the MD with data (and pay attention to other comments under "part 1", above).

Yes. Please see our reply to the last comment in Part 1.

3) When revising what we have called "part 2", comply with each of the three paragraphs under "part 2", above.

Yes. Please see our replies to the comments in Part 2 above.

4) Provide details (in the Methods) for the nonlinear least-square fitting that converts dwell times to deltaG (or deltaG double dagger).

Yes, we have provided details in Methods for the nonlinear least-square fitting to derive the energies of intermediate states and transition states.

[Editors' note: further revisions were requested prior to acceptance, as described below.]

Essential revisions:

A) The subsection entitled "Position-dependent effects of layer mutation on SNARE assembly", in which the authors discuss single-molecule mechanics of 15 SNARE complex mutants, was very difficult to follow. We propose the following changes: 1) In Figure 4, show explicitly the name of the domain (NTD, MTD and CTD) to which each mutant belongs.

Following the reviewers’ suggestion, we have explicitly shown the name of the domain to which each mutant belongs. In addition, we have color-coded the mutation names to blue, green, and red based on their associated NTD, MD, and CTD, respectively. The same color-coding is applied to mutation names in Figures 5 and 6 and Figure 5—figure supplement 1, 2.

2) In the same figure, the current way in which FECs are marked is difficult to recognize. The colors and patterns are too similar. One way is to depict the corresponding transitions right next to individual FEC regions.

We have improved the labeling by adding domain names next to the corresponding transitions in FECs, as the reviewers suggested. In addition, we have simplified the labeling by only showing the abnormal transitions of the mutant SNARE complexes compared to the wild-type.

3) How is "MD+NTD" different from "MD_NTD"? The reviewers could not find proper explanations neither in the main text nor figure legends.

The “MD+NTD” transition means sequential MD and NTD transitions in an overlapping force range, whereas the “MD_NTD” transition indicates two-state transition of MD and NTD as a combined new domain. To address the reviewers’ concern, we have added Figure 4—figure supplement 1 to illustrate the change in SNARE folding pathway. In addition, we have clarified our nomenclature in several places in the main text, as well as in the legend to Figure 4.

4) In Figure 5, each mutant trace is labeled with jargon, such as, "M46A CTD+MD_NTD". This labeling is nearly impossible to understand. It may be enough to depict the corresponding domains above the subpanel of Figure 5B (i.e., LC, CTD, MD and NTD). And the readers can then interpret the data as they are.

As is described in our reply to the preceding question, we have depicted the difference between sequential transitions and cooperative transitions in Figure 4—figure supplement 1, using “MD+NTD” and “MD_NTD” as an example. Combining with our clarified definition of the nomenclature in the main text, we think the nomenclature can be better understood. These nomenclatures are well consistent with our labeling of different state positions in the extension-time trajectories (Figure 5).

b) Figure 11 is also hard to follow. The authors introduced new States 10 and 11. Observation of the State 11 was attributed to folding of the C-terminal end of the t-SNARE proteins (called Tc in the manuscript) induced by Munc18-1 binding. An immediate question is whether such Tc structuring was observed in the presence of NRD. Also, the authors argued that the two partially-zipped states, State 9 and State 10, are different from each other (subsection “Munc18-1 induces t-SNARE folding”), which the reviewers could not understand. Because the NRD-truncated SNARE complex has less biological relevance, the authors may want consider moving Figure 11 to supplementary data. The data in Figures 9, 10, 12 and 13 collectively make a smooth flow, but the data in Figure 11 seem at odds with those in the other figures.

We thank the reviewers for pointing out our confusing description regarding Figure 11. We have made significant revision in this part to address the reviewers’ comments. First, the Tc structuring was indeed observed in the presence of NRD, although with much lower probability than in the absence of NRD. We have added Figure 11—figure supplement 3 to show Munc18-1-induced folding of Tc in the SNARE complex containing NRD. Second, we agree with the reviewers that our original description on the difference between state 9 and state 10 is confusing. We have revised the relevant sentences. Basically, the two states differ in their Munc18-1 binding sites on the SNARE complex, the VAMP2 zippering states, and mechanical stabilities. Third, we have added a few sentences at the beginning of the section to rationalize the experiments described in this section and emphasize their biological relevance. Previous experiments show that, although the NRD is initially required to recruit Munc18-1 to bind the trans-SNARE complex, the NRD becomes dispensable for the subsequent membrane fusion, indicating the existence of an NRD-independent Munc18-1-SNARE binding mode. The NRD-independent, Munc18-1-mediated Tc folding discovered by us is consistent with the predicted binding mode. We believe this binding mode is important, because it shares the same mechanism by which Vc and Vn peptides enhances SNARE-mediated membrane fusion in vitro. Based on these thoughts and our clarifications, we kept Figure 11 as a main figure. In addition, this figure strengthens our argument for multiple Munc18-1 binding modes and their roles in SNARE assembly and membrane fusion depicted in Figure 14.


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