Homotypic fusion of early endosomes: SNAREs do not determine fusion specificity

Brandhorst, Dorothea; Zwilling, Daniel; Rizzoli, Silvio O.; Lippert, Undine; Lang, Thorsten; Jahn, Reinhard

doi:10.1073/pnas.0511138103

Cited by 130 publications

(193 citation statements)

References 57 publications

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“…In contrast, the other conclusion provides the quite divergent concept that SNARE pairing is rather promiscuous and, thereby, largely incapable of regulating fusion specificity. Indeed, in vitro experiments with SNAREs in mammals showed that the endosomal and exocytic SNAREs readily form noncognate and mixed SNARE complexes (43,44) and cause promiscuous RPL fusion by non-physiological SNARE pairing (24). Despite the fact that we used the same approaches with the purified SNAREs and the RPL lipid mixing assay, our conclusions do not fully agree with either of these previous concepts.…”

Section: Discussioncontrasting

confidence: 54%

“…Despite the fact that we used the same approaches with the purified SNAREs and the RPL lipid mixing assay, our conclusions do not fully agree with either of these previous concepts. This might be due to the differences in experimental details, including lipid compositions, lipid to protein ratios, and salt concentrations (22,24). Nevertheless, our findings establish that Q-SNAREs are the key components to mediate fusion specificity through the specific assembly of appropriate Qabc-SNARE complexes, whereas R-SNAREs have little contribution.…”

Section: Discussionmentioning

confidence: 77%

“…This RPL approach has been further employed to test whether SNAREs themselves ensure the specificity of membrane fusion (22)(23)(24). A high degree of specificity was observed by comprehensive analyses with yeast SNAREs (22), whereas RPLs bearing mammalian SNAREs in the endosomal and exocytic pathways can fuse rather promiscuously (24).…”

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confidence: 99%

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Distinct Contributions of Vacuolar Qabc- and R-SNARE Proteins to Membrane Fusion Specificity

Izawa

Onoue

Furukawa

et al. 2012

Journal of Biological Chemistry

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Background: Qabc-and R-SNARE proteins are key components for membrane fusion in eukaryotic organelles. Results: Reconstituted SNARE proteoliposomal study reveals distinct contributions of Qabc-and R-SNAREs to the specificity of membrane fusion. Conclusion: An assembly of proper Qabc-SNARE combinations is critical for mediating fusion specificity. Significance: This provides new insights for understanding how cells organize their complex membrane trafficking pathways.

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Section: Discussioncontrasting

confidence: 54%

Section: Discussionmentioning

confidence: 77%

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Distinct Contributions of Vacuolar Qabc- and R-SNARE Proteins to Membrane Fusion Specificity

Izawa

Onoue

Furukawa

et al. 2012

Journal of Biological Chemistry

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“…The expression constructs for the neuronal SNAREs were the full-length syntaxin-1A (amino acid residues 1-288), its SNARE motif including the transmembrane region (183-288), a cysteine-free variant of SNAP-25A (1-206) and synaptobrevin-2 (full-length protein, 1-116; soluble portion, 1-96; C-terminal fragment of the soluble portion, 49-96) 30,39,45,46 . The expression constructs for endobrevin were the full-length protein (1-100) and its soluble portion (1-74) 46,47 . Full-length syntaxin-4 (1-298) 48 and a variant of SNAP-23 in which cysteine residues were replaced with serines were similarly cloned into the pET28a vector using the NdeI and XhoI restriction sites.…”

Section: Methodsmentioning

confidence: 99%

Synaptotagmin activates membrane fusion through a Ca2+-dependent trans interaction with phospholipids

Stein

Radhakrishnan

Riedel

et al. 2007

Nat Struct Mol Biol

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164

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Synaptotagmin-1 is the calcium sensor for neuronal exocytosis, but the mechanism by which it triggers membrane fusion is not fully understood. Here we show that synaptotagmin accelerates SNARE-dependent fusion of liposomes by interacting with neuronal Q-SNARES in a Ca 2+ -independent manner. Ca 2+ -dependent binding of synaptotagmin to its own membrane impedes the activation. Preventing this cis interaction allows Ca 2+ to trigger synaptotagmin binding in trans, accelerating fusion. However, when an activated SNARE acceptor complex is used, synaptotagmin has no effect on fusion kinetics, suggesting that synaptotagmin operates upstream of SNARE assembly in this system. Our results resolve major discrepancies concerning the effects of full-length synaptotagmin and its C2AB fragment on liposome fusion and shed new light on the interactions of synaptotagmin with SNAREs and membranes. However, our findings also show that the action of synaptotagmin on the fusionarrested state of docked vesicles in vivo is not fully reproduced in vitro.Neurotransmitters are stored in synaptic vesicles that undergo Ca 2+ -dependent exocytosis upon stimulation. Fusion of synaptic vesicles with the presynaptic plasma membrane is mediated by the neuronal soluble N-ethylmaleimide-sensitive factor attachment protein (SNAP) receptor (SNARE) proteins, including synaptobrevin-2 (also referred to as VAMP2) in the membrane of synaptic vesicles and syntaxin-1 and SNAP-25 in the plasma membrane. SNAREs are characterized by conserved stretches of 60-70 amino acid residues, referred to as SNARE motifs. Syntaxin-1 and synaptobrevin-2 each possess a single SNARE motif adjacent to the C-terminal transmembrane domain, whereas SNAP-25 contains two SNARE motifs that are separated by a palmitoylated linker 1,2 . The SNARE motifs are unstructured as monomers 3 but assemble into a tight bundle of four a-helices 4 . SNARE motifs are divided into four conserved subfamilies, referred to as Qa-, Qb-, Qc-and R-SNARE motifs. Each SNARE complex contains one member of each subfamily 5 . The assembly of SNARE complexes is currently believed to be the essential reaction in driving membrane fusion. According to this model, the formation of the SNARE complex is initiated in a trans configuration at the N-terminal ends of the SNARE motifs, forming a bridge between the membranes. Assembly then proceeds toward the C-terminal membrane anchor domains, clamping the membranes together and thus overcoming the energy barrier for fusion [6][7][8] .In contrast to several other SNARE-dependent fusion reactions, neuronal exocytosis is strongly upregulated by calcium 9 . The fast component of Ca 2+ -dependent release, which is essential for synchronous, action potential-coupled release, is mediated by the proteins synaptotagmin-1, synaptotagmin-2 and probably synaptotagmin-9, which reside in the membrane of synaptic vesicles 2 . Synaptotagmins constitute a family of type I membrane proteins with widespread tissue distribution 10 . The cytoplasmic part of the synaptotagmins contains t...

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“…One of the reasons for this gap in our knowledge is that, in contrast to fusion (3,4), it has been difficult to reconstitute sorting from endosomes in vitro. Compared to live cell approaches, in vitro assays allow direct biochemical access to the docking and fusion machineries (for instance, proteins can be depleted or perturbed using cell-impermeant inhibitors such as antibodies).…”

mentioning

confidence: 99%

Sorting in early endosomes reveals connections to docking- and fusion-associated factors

Barysch

Aggarwal

Jahn

et al. 2009

Proc. Natl. Acad. Sci. U.S.A.

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The early endosomes constitute a major sorting platform in eukaryotic cells. They receive material through fusion with endocytotic vesicles or with trafficking vesicles from the Golgi complex and later sort it into budding vesicles. While endosomal fusion is well understood, sorting is less characterized; the 2 processes are generally thought to be effected by different, unrelated machineries. We developed here a cell-free assay for sorting/budding from early endosomes, by taking advantage of their ability to segregate different cargoes (such as transferrin, cholera toxin subunit B, and low-density lipoprotein, LDL) into different carrier vesicles. Cargo separation required both carrier vesicle formation and active maturation of the endosomes. Sorting and budding were insensitive to reagents perturbing clathrin coats, coatomer protein complex-I (COPI) coats, dynamin, and actin, but were inhibited by anti-retromer subunit antibodies. In addition, the process required Rab-GTPases, phosphatidylinositol-3-phosphate, and, surprisingly, the docking factor early endosomal autoantigen 1 (EEA1). Sorting also required the function of the N-ethylmaleimide-sensitive factor (NSF), a well-known fusion cofactor, while it did not depend on preceding fusion of endosomes. We conclude that fusion, docking, and sorting/budding are interconnected at the molecular level.budding ͉ EEA1 ͉ in vitro ͉ NSF ͉ SNAREs

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Homotypic fusion of early endosomes: SNAREs do not determine fusion specificity

Cited by 130 publications

References 57 publications

Distinct Contributions of Vacuolar Qabc- and R-SNARE Proteins to Membrane Fusion Specificity

Distinct Contributions of Vacuolar Qabc- and R-SNARE Proteins to Membrane Fusion Specificity

Synaptotagmin activates membrane fusion through a Ca2+-dependent trans interaction with phospholipids

Sorting in early endosomes reveals connections to docking- and fusion-associated factors

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