Literature DB >> 30456600

BAR domain proteins-a linkage between cellular membranes, signaling pathways, and the actin cytoskeleton.

Peter J Carman1,2, Roberto Dominguez3,4.   

Abstract

Actin filament assembly typically occurs in association with cellular membranes. A large number of proteins sit at the interface between actin networks and membranes, playing diverse roles such as initiation of actin polymerization, modulation of membrane curvature, and signaling. Bin/Amphiphysin/Rvs (BAR) domain proteins have been implicated in all of these functions. The BAR domain family of proteins comprises a diverse group of multi-functional effectors, characterized by their modular architecture. In addition to the membrane-curvature sensing/inducing BAR domain module, which also mediates antiparallel dimerization, most contain auxiliary domains implicated in protein-protein and/or protein-membrane interactions, including SH3, PX, PH, RhoGEF, and RhoGAP domains. The shape of the BAR domain itself varies, resulting in three major subfamilies: the classical crescent-shaped BAR, the more extended and less curved F-BAR, and the inverse curvature I-BAR subfamilies. Most members of this family have been implicated in cellular functions that require dynamic remodeling of the actin cytoskeleton, such as endocytosis, organelle trafficking, cell motility, and T-tubule biogenesis in muscle cells. Here, we review the structure and function of mammalian BAR domain proteins and the many ways in which they are interconnected with the actin cytoskeleton.

Entities:  

Keywords:  Actin cytoskeleton; BAR domain; Membrane remodeling; Rho GTPases; Signaling

Year:  2018        PMID: 30456600      PMCID: PMC6297083          DOI: 10.1007/s12551-018-0467-7

Source DB:  PubMed          Journal:  Biophys Rev        ISSN: 1867-2450


  197 in total

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3.  The N terminus of amphiphysin II mediates dimerization and plasma membrane targeting.

Authors:  A R Ramjaun; J Philie; E de Heuvel; P S McPherson
Journal:  J Biol Chem       Date:  1999-07-09       Impact factor: 5.157

4.  Bin2, a functionally nonredundant member of the BAR adaptor gene family.

Authors:  K Ge; G C Prendergast
Journal:  Genomics       Date:  2000-07-15       Impact factor: 5.736

5.  Rvs161p and Rvs167p, the two yeast amphiphysin homologs, function together in vivo.

Authors:  R Lombardi; H Riezman
Journal:  J Biol Chem       Date:  2000-11-28       Impact factor: 5.157

6.  Functional partnership between amphiphysin and dynamin in clathrin-mediated endocytosis.

Authors:  K Takei; V I Slepnev; V Haucke; P De Camilli
Journal:  Nat Cell Biol       Date:  1999-05       Impact factor: 28.824

7.  Rho small G-protein-dependent binding of mDia to an Src homology 3 domain-containing IRSp53/BAIAP2.

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8.  The structural basis of Arfaptin-mediated cross-talk between Rac and Arf signalling pathways.

Authors:  C Tarricone; B Xiao; N Justin; P A Walker; K Rittinger; S J Gamblin; S J Smerdon
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9.  Syndapin isoforms participate in receptor-mediated endocytosis and actin organization.

Authors:  B Qualmann; R B Kelly
Journal:  J Cell Biol       Date:  2000-03-06       Impact factor: 10.539

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Authors:  J Modregger; B Ritter; B Witter; M Paulsson; M Plomann
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  38 in total

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2.  Membrane curvature underlies actin reorganization in response to nanoscale surface topography.

Authors:  Hsin-Ya Lou; Wenting Zhao; Xiao Li; Liting Duan; Alexander Powers; Matthew Akamatsu; Francesca Santoro; Allister F McGuire; Yi Cui; David G Drubin; Bianxiao Cui
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5.  Light Scattering Techniques to Assess Self-Assembly and Hydrodynamics of Membrane Trafficking Proteins.

Authors:  Marijn G J Ford; Rajesh Ramachandran
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6.  IRSp53 promotes postsynaptic density formation and actin filament bundling.

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7.  The adaptor protein APPL2 controls glucose-stimulated insulin secretion via F-actin remodeling in pancreatic β-cells.

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8.  BIN2 orchestrates platelet calcium signaling in thrombosis and thrombo-inflammation.

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Review 9.  Structure and regulation of phospholipase Cβ and ε at the membrane.

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10.  CryoEM reveals BIN1 (isoform 8) does not bind to single actin filaments in vitro.

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