Literature DB >> 19161383

Identifying critical components of native Ca2+-triggered membrane fusion. Integrating studies of proteins and lipids.

Kendra L Furber1, Matthew A Churchward, Tatiana P Rogasevskaia, Jens R Coorssen.   

Abstract

Ca(2+)-triggered membrane fusion is the defining step of exocytosis. Despite realization that the fusion machinery must include lipids and proteins working in concert, only of late has work in the field focused more equally on both these components. Here we use isolated sea urchin egg cortical vesicles (CV), a stage-specific preparation of Ca(2+)-sensitive release-ready vesicles that enables the tight coupling of molecular and functional analyses necessary to dissect molecular mechanisms. The stalk-pore hypothesis proposes that bilayer merger proceeds rapidly via transient, high-negative curvature, intermediate membrane structures. Consistent with this, cholesterol, a major component of the CV membrane, contributes to a critical local negative curvature that supports formation of lipidic fusion intermediates. Following cholesterol depletion, structurally dissimilar lipids having intrinsic negative curvature greater than or equal to cholesterol recover the ability of CV to fuse but do not recover fusion efficiency (Ca(2+) sensitivity and kinetics). Conversely, cholesterol- and sphingomyelin-enriched microdomains regulate the efficiency of the fusion mechanism, presumably by contributing spatial and functional organization of other critical lipids and proteins at the fusion site. Critical proteins are thought to participate in Ca(2+) sensing, initiating membrane deformations, and facilitating fusion pore expansion. Capitalizing on a novel effect of the thiol-reactive reagent iodoacetamide (IA), potentiation of the Ca(2+) sensitivity and kinetics, a fluorescently tagged IA has been used to enhance fusion efficiency and simultaneously label the proteins involved. Isolation of cholesterol-enriched CV membrane fractions, using density gradient centrifugation, is being used to narrow the list of protein candidates potentially critical to the mechanism of fast Ca(2+)-triggered membrane fusion.

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Year:  2009        PMID: 19161383     DOI: 10.1111/j.1749-6632.2008.03993.x

Source DB:  PubMed          Journal:  Ann N Y Acad Sci        ISSN: 0077-8923            Impact factor:   5.691


  7 in total

1.  A new approach to the molecular analysis of docking, priming, and regulated membrane fusion.

Authors:  Tatiana P Rogasevskaia; Jens R Coorssen
Journal:  J Chem Biol       Date:  2011-02-08

Review 2.  Lipid dynamics in exocytosis.

Authors:  S Chasserot-Golaz; J R Coorssen; F A Meunier; N Vitale
Journal:  Cell Mol Neurobiol       Date:  2010-11-16       Impact factor: 5.046

Review 3.  Mechanism of Membrane Fusion: Interplay of Lipid and Peptide.

Authors:  Ankita Joardar; Gourab Prasad Pattnaik; Hirak Chakraborty
Journal:  J Membr Biol       Date:  2022-04-18       Impact factor: 2.426

4.  Combined targeted Omic and Functional Assays Identify Phospholipases A₂ that Regulate Docking/Priming in Calcium-Triggered Exocytosis.

Authors:  Deepti Dabral; Jens R Coorssen
Journal:  Cells       Date:  2019-04-02       Impact factor: 6.600

5.  Chronic palmitate exposure inhibits insulin secretion by dissociation of Ca(2+) channels from secretory granules.

Authors:  Michael B Hoppa; Stephan Collins; Reshma Ramracheya; Leanne Hodson; Stefan Amisten; Quan Zhang; Paul Johnson; Frances M Ashcroft; Patrik Rorsman
Journal:  Cell Metab       Date:  2009-12       Impact factor: 27.287

6.  Application of High-Throughput Assays to Examine Phospho-Modulation of the Late Steps of Regulated Exocytosis.

Authors:  Prabhodh S Abbineni; Jens R Coorssen
Journal:  High Throughput       Date:  2017-11-13

7.  Unbiased Thiol-Labeling and Top-Down Proteomic Analyses Implicate Multiple Proteins in the Late Steps of Regulated Secretion.

Authors:  Kendra L Furber; Peter S Backlund; Alfred L Yergey; Jens R Coorssen
Journal:  Proteomes       Date:  2019-09-27
  7 in total

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