Munc13 proteins are essential in neurotransmitter release, controlling the priming of synaptic vesicles to a release-ready state. The sequences responsible for this priming activity are unknown. Here we identify a large alpha-helical domain of mammalian Munc13-1 that is autonomously folded and is sufficient to rescue the total arrest in neurotransmitter release observed in hippocampal neurons lacking Munc13s.
The Ly49 family of natural killer (NK) receptors regulates NK cell function by sensing major histocompatibility complex (MHC) class I. Ly49 receptors show complex patterns of MHC class I cross-reactivity and, in certain cases, peptide selectivity. To investigate whether specificity differences result from topological differences in MHC class I engagement, we determined the structure of the peptide-selective receptor Ly49C in complex with H-2K(b). The Ly49C homodimer binds two MHC class I molecules in symmetrical way, a mode distinct from that of Ly49A, which binds MHC class I asymmetrically. Ly49C does not directly contact the MHC-bound peptide. In addition, MHC crosslinking by Ly49C was demonstrated in solution. We propose a dynamic model for Ly49-MHC class I interactions involving conformational changes in the receptor, whereby variations in Ly49 dimerization mediate different MHC-binding modes.
Structural basis for peptidoglycan binding by peptidoglycan recognition proteins
Peptidoglycan (PGN) recognition proteins (PGRPs) are patternrecognition receptors of the innate immune system that bind and, in some cases, hydrolyze bacterial PGNs. We determined the crystal structure, at 2.30-Å resolution, of the C-terminal PGN-binding domain of human PGRP-I␣ in complex with a muramyl tripeptide representing the core of lysine-type PGNs from Gram-positive bacteria. The peptide stem of the ligand is buried at the deep end of a long binding groove, with N-acetylmuramic acid situated in the middle of the groove, whose shallow end can accommodate a linked N-acetylglucosamine. Although most interactions are with the peptide, the glycan moiety also seems to be essential for specific recognition by PGRPs. Conservation of key PGN-contacting residues shows that all PGRPs employ this basic PGN-binding mode. The structure pinpoints variable residues that likely mediate discrimination between lysine-and diaminopimelic acid-type PGNs. We also propose a mechanism for PGN hydrolysis by Zn 2؉ -containing PGRPs.innate immunity ͉ bacteria ͉ receptor ͉ complex ͉ crystal structure
Active sites and ligand binding cavities in native proteins are often formed by curved β-sheets, and the ability to control β-sheet curvature would allow design of binding proteins with cavities customized to specific ligands. Towards this end, we investigated the mechanisms controlling β-sheet curvature by studying the geometry of β-sheets in naturally occurring protein structures and * Correspondence to: dabaker@u.washington.edu. † These authors contributed equally to this work. Supplementary Materials: Materials and MethodsFigs. S1 to S22 Tables S1 to S7 Input files and command lines for design calculations HHS Public Access Author Manuscript Author ManuscriptAuthor ManuscriptAuthor Manuscript folding simulations. The principles emerging from this analysis were used to de novo design a series of proteins with curved β-sheets topped with a-helices. NMR and crystal structures of the designs closely match the computational models, showing that β-sheet curvature can be controlled with atomic-level accuracy. Our approach enables the design of proteins with cavities and provides a route to custom design ligand binding and catalytic sites.Ligand binding proteins with curved β-sheets surrounding the binding pocket, as in the NTF2-like, β-barrel, and jelly roll folds, play key roles in molecular recognition, metabolic pathways and cell signaling. Approaches to designing small molecule binding proteins and enzymes to date have started by searching for native protein scaffolds with ligand binding pockets with roughly the right geometry, and then redesigning the surrounding residues to optimize interactions with the small molecule. While this approach has yielded new binding proteins and catalysts (1-5), it is not optimal: there may be no naturally occurring scaffold with a pocket with the correct geometry, and introduction of mutations in the design process may change the pocket structure (6, 7). Building de novo proteins with custom-tailored binding sites could be a more effective strategy, but this remains an outstanding challenge (8-11). De novo protein design has recently focused on proteins with ideal backbone structures (12-16) (straight helices, uniform β-strands and short loops; see ref (17) for a recent exception) and optimal core sidechain packing, but the binding pockets of naturally occurring proteins lie on concave surfaces formed by non-ideal features such as kinked helices, curved β-sheets or long loops. The design of proteins with concave surfaces requires examination of how such irregular structural features can be programmed into the amino acid sequence.We begin by analyzing how classic (18, 19) β-bulges (irregularities in the pleating of edge strands) and register shifts (local termination of strand pairing) coupled with intrinsic β-strand geometry induce curvature in antiparallel β-sheets (20, 21). We quantify the curvature of an edge strand making an antiparallel pairing with a second strand by the bend angle (Fig. 1A). The absolute value of the bend angle (α) at residue i is the angle bet...
The core of the membrane fusion machinery that governs neurotransmitter release includes the SNARE proteins syntaxin-1, SNAP-25 and synaptobrevin, which form a tight "SNARE complex", and Munc18-1, which binds to the SNARE complex and to syntaxin-1 folded into a closed conformation. Release is also controlled by specialized proteins such as complexins, which also bind to the SNARE complex, and unc13/Munc13s, which are crucial for synaptic vesicle priming and were proposed to open syntaxin-1, promoting SNARE complex assembly. However, the biochemical basis for unc13/Munc13 function and its relationship to other SNARE interactions are unclear. To address this question, we have analyzed interactions of the MUN domain of Munc13-1, which is key for this priming function, using solution binding assays and cofloatation experiments with SNARE-containing proteoliposomes. Our results indicate that the Munc13-1 MUN domain binds to membrane-anchored SNARE complexes, even though binding is barely detectable in solution. The MUN domain appears to compete with Munc18-1 but not with complexin-1 for SNARE complex binding, although more quantitative assays will be required to verify these conclusions. Moreover, our data also uncover interactions of membrane-anchored syntaxin-1/SNAP-25 heterodimers with the MUN domain, Munc18-1 and complexin-1. The interaction with complexin-1 is surprising, as it was not observed in previous solution studies. Our results emphasize the importance of studying interactions within the neurotransmitter release machinery in a native membrane environment, and suggest that unc13/Munc13s may provide a template to assemble syntaxin-1/SNAP-25 heterodimers, leading to an acceptor complex for synaptobrevin.
Dual strategies for peptidoglycan discrimination by peptidoglycan recognition proteins (PGRPs)
The innate immune system constitutes the first line of defense against microorganisms in both vertebrates and invertebrates. Although much progress has been made toward identifying key receptors and understanding their role in host defense, far less is known about how these receptors recognize microbial ligands. Such studies have been severely hampered by the need to purify ligands from microbial sources and a reliance on biological assays, rather than direct binding, to monitor recognition. We used synthetic peptidoglycan (PGN) derivatives, combined with microcalorimetry, to define the binding specificities of human and insect peptidogycan recognition proteins (PGRPs). We demonstrate that these innate immune receptors use dual strategies to distinguish between PGNs from different bacteria: one based on the composition of the PGN peptide stem and another that senses the peptide bridge crosslinking the stems. To pinpoint the site of PGRPs that mediates discrimination, we engineered structure-based variants having altered PGN-binding properties. The plasticity of the PGRPbinding site revealed by these mutants suggests an intrinsic capacity of the innate immune system to rapidly evolve specificities to meet new microbial challenges.affinity ͉ bacteria ͉ innate immunity ͉ calorimetry ͉ synthesis T he innate immune system recognizes invading microbes by means of conserved pattern recognition receptors that bind unique products of microbial metabolism not produced by the host (pathogen-associated molecular patterns) (1, 2). Examples of microbial ligands recognized by pattern recognition receptors such as Toll-like receptors, peptidoglycan recognition proteins (PGRPs), and NOD proteins include lipopolysaccharide of Gram-negative bacteria, lipoteichoic acid of Gram-positive bacteria, nonmethylated CpG sequences, flagellin, and peptidoglycan (PGN) of Gram-negative and -positive bacteria. Cellular activation by pattern recognition receptors results in acute inflammatory responses involving cytokine and chemokine production, direct local attack against the invading pathogen, and induction of the adaptive component of the immune system. In humans, overactivation of inflammatory responses can lead to septic shock, which accounts for 100,000 deaths annually in the United States alone. By sitting at the intersection of the pathways of microbial recognition, inflammation, and cell death, the innate immune system offers emerging opportunities for the development of therapeutics to modulate immune responses (3).PGRPs, a newly discovered class of pattern recognition receptors, are highly conserved from insects to mammals (4-7). By detecting PGN from both Gram-negative and -positive bacteria, PGRPs are important contributors to host defense against microbial infections (2, 4). PGNs are polymers of alternating Nacetylglucosamine (GlcNAc) and N-acetylmuramic acid (MurNAc) in (134) linkage, crosslinked by short peptide stems composed of alternating L-and D-amino acids (8, 9) (Fig. 1A). Whereas the carbohydrate backbone is conserved a...
SUMMARY Unc13/Munc13s play a crucial function in neurotransmitter release through their MUN domain, which mediates the transition from the syntaxin-1/Munc18-1 complex to the SNARE complex. The MUN domain was suggested to be related to tethering factors, but no MUN-domain structure is available to experimentally validate this notion and address key unresolved questions about the interactions and minimal structural unit required for Unc13/Munc13 function. Here we identify an autonomously folded module within the MUN domain (MUN-CD) and show that its crystal structure is remarkably similar to several tethering factors. We also show that the activity in promoting the syntaxin-1/Munc18-1 to SNARE complex transition is strongly impaired in MUN-CD. These results show that MUN domains and tethering factors indeed belong to the same family and may have a common role in membrane trafficking, and suggest a model whereby the MUN-CD module is central for Munc13 function but full activity requires adjacent sequences.
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