A Role for Soluble <i>N</i>-Ethylmaleimide-sensitive Factor Attachment Protein Receptor Complex Dimerization during Neurosecretion

Fdez, Elena; Jowitt, Thomas A.; Wang, Ming Chuan; Rajebhosale, Manisha; Foster, Keith A.; Bella, Jordi; Baldock, Clair; Woodman, Philip; Hilfiker, Sabine

doi:10.1091/mbc.e08-01-0010

Cited by 13 publications

(17 citation statements)

References 56 publications

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“…For this purpose, neuroendocrine PC12 cells were transfected with a plasmid containing both non-tagged VAMP2 and human growth hormone (hGH) (Fdez et al, 2008). Cells were permeabilised and treated with recombinant botulinum neurotoxin type F light-chain (botF/LC), which cleaves and inactivates VAMP2 (Fig.…”

Section: Tmd-mediated Vamp2 Interactions Are Not Important For Neurosmentioning

confidence: 99%

“…For secretion assays, full-length, non-tagged rat VAMP2 (residues 1-116) was expressed from a pCMV-driven promoter in a vector where expression of hGH is driven from an SV40 promoter (pCMV5-VAMP2-SV40-hGH) (Fdez et al, 2008). C-terminally GFP-tagged VAMP2 was generated by subcloning full-length VAMP2 into a pGFPemd vector (Packard) using the EcoRI-BamHI sites, with a resulting linker (TDPPVAT) between the VAMP2 and the GFP sequences.…”

Section: Plasmid Constructs and Site-directed Mutagenesismentioning

confidence: 99%

“…PC12 cells were grown and transfected essentially as described (Fdez et al, 2008). Double transfections were performed with each 2.4 g DNA using 10 l LipofectAMINE 2000 (Invitrogen).…”

Section: Pc12 Cell Culture Transfection and Imagingmentioning

confidence: 99%

“…Cells were examined either live, or upon fixation (Fdez et al, 2008) and mounting (ProLong-Gold antifade reagent, Invitrogen). For colocalisation analysis, the following antibodies were used: rabbit polyclonal antisynaptotagmin (p65, 1:1000) (Fdez et al, 2008), mouse monoclonal anti-VAMP2 (Cl 69.1, Synaptic Systems, 1:5000), mouse monoclonal anti-rat TGN38 (BD Biosciences, 1:800), rabbit polyclonal anti-calnexin (Stressgen, SPA860, 1:300), mouse monoclonal anti-syntaxin-(CL HPC-1, SIGMA, 1:500), mouse monoclonal anti-TfR (Invitrogen, 1:300), mouse monoclonal anti-EEA1 (BD Biosciences, 1:250), mouse monoclonal anti-synaptophysin (CL SVP38, Sigma, 1:200), mouse monoclonal anti-GM130 (BD Biosciences, 1:100) and rabbit polyclonal anti-GFP (Abcam, 1:500). Secondary antibodies included Alexa Fluor 594-conjugated goat anti-mouse (Invitrogen, 1:1000) and Alexa Fluor 594-conjugated goat anti-rabbit (Invitrogen, 1:1000).…”

Section: Pc12 Cell Culture Transfection and Imagingmentioning

confidence: 99%

“…Distinct molecular interactions responsible for oligomerisation of SNARE complexes have been reported (Littleton et al, 2001;Tokumaru et al, 2001;Kweon et al, 2002;Rickman et al, 2005;Fdez et al, 2008), including interactions mediated by the transmembrane domains (TMDs). For example, self-interaction of the syntaxin-1A TMDs has been proposed to have a scaffolding role for the subsequent formation of a supramolecular SNARE complex at the fusion site (Lu et al, 2008), or to be implicated in mediating the transition from a hemifusion to a full-fusion state (Hofmann et al, 2006).…”

Section: Introductionmentioning

confidence: 99%

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Transmembrane-domain determinants for SNARE-mediated membrane fusion

Fdez

Martínez-Salvador

Beard

et al. 2010

Journal of Cell Science

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SummaryNeurosecretion involves fusion of vesicles with the plasma membrane. Such membrane fusion is mediated by the SNARE complex, which is composed of the vesicle-associated protein synaptobrevin (VAMP2), and the plasma membrane proteins syntaxin-1A and SNAP-25. Although clearly important at the point of membrane fusion, the precise structural and functional requirements for the transmembrane domains (TMDs) of SNAREs in bringing about neurosecretion remain largely unknown. Here, we used a bimolecular fluorescence complementation (BiFC) approach to study SNARE protein interactions involving TMDs in vivo. VAMP2 molecules were found to dimerise through their TMDs in intact cells. Dimerisation was abolished when replacing a glycine residue in the centre of the TMD with residues of increasing molecular volume. However, such mutations still were fully competent in bringing about membrane-fusion events, suggesting that dimerisation of the VAMP2 TMDs does not have an important functional role. By contrast, a series of deletion or insertion mutants in the C-terminal half of the TMD were largely deficient in supporting neurosecretion, whereas mutations in the N-terminal half did not display severe secretory deficits. Thus, structural length requirements, largely confined to the C-terminal half of the VAMP2 TMD, seem to be essential for SNARE-mediated membrane-fusion events in cells.

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Section: Tmd-mediated Vamp2 Interactions Are Not Important For Neurosmentioning

confidence: 99%

Section: Plasmid Constructs and Site-directed Mutagenesismentioning

confidence: 99%

Section: Pc12 Cell Culture Transfection and Imagingmentioning

confidence: 99%

Section: Pc12 Cell Culture Transfection and Imagingmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Transmembrane-domain determinants for SNARE-mediated membrane fusion

Fdez

Martínez-Salvador

Beard

et al. 2010

Journal of Cell Science

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V-ATPase Membrane Sector Associates with Synaptobrevin to Modulate Neurotransmitter Release

Giovanni

Boudkkazi

Mochida

et al. 2010

Neuron

115

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Acidification of synaptic vesicles by the vacuolar proton ATPase is essential for loading with neurotransmitter. Debated findings have suggested that V-ATPase membrane domain (V0) also contributes to Ca(2+)-dependent transmitter release via a direct role in vesicle membrane fusion, but the underlying mechanisms remain obscure. We now report a direct interaction between V0 c-subunit and the v-SNARE synaptobrevin, constituting a molecular link between the V-ATPase and SNARE-mediated fusion. Interaction domains were mapped to the membrane-proximal domain of VAMP2 and the cytosolic 3.4 loop of c-subunit. Acute perturbation of this interaction with c-subunit 3.4 loop peptides did not affect synaptic vesicle proton pump activity, but induced a substantial decrease in neurotransmitter release probability, inhibiting glutamatergic as well as cholinergic transmission in cortical slices and cultured sympathetic neurons, respectively. Thus, V-ATPase may ensure two independent functions: proton transport by a fully assembled V-ATPase and a role in SNARE-dependent exocytosis by the V0 sector.

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