Literature DB >> 8647895

Filensin and phakinin form a novel type of beaded intermediate filaments and coassemble de novo in cultured cells.

G Goulielmos1, F Gounari, S Remington, S Müller, M Häner, U Aebi, S D Georgatos.   

Abstract

The fiber cells of the eye lens possess a unique cytoskeletal system known as the "beaded-chain filaments" (BFs). BFs consist of filensin and phakinin, two recently characterized intermediate filament (IF) proteins. To examine the organization and the assembly of these heteropolymeric IFs, we have performed a series of in vitro polymerization studies and transfection experiments. Filaments assembled from purified filensin and phakinin exhibit the characteristic 19-21-nm periodicity seen in many types of IFs upon low angle rotary shadowing. However, quantitative mass-per-length (MPL) measurements indicate that filensin/phakinin filaments comprise two distinct and dissociable components: a core filament and a peripheral filament moiety. Consistent with a nonuniform organization, visualization of unfixed and unstained specimens by scanning transmission electron microscopy (STEM) reveals the the existence of a central filament which is decorated by regularly spaced 12-15-nm-diam beads. Our data suggest that the filamentous core is composed of phakinin, which exhibits a tendency to self-assemble into filament bundles, whereas the beads contain filensin/phakinin hetero-oligomers. Filensin and phakinin copolymerize and form filamentous structures when expressed transiently in cultured cells. Experiments in IF-free SW13 cells reveal that coassembly of the lens-specific proteins in vivo does not require a preexisting IF system. In epithelial MCF-7 cells de novo forming filaments appear to grow from distinct foci and organize as thick, fibrous laminae which line the plasma membrane and the nuclear envelope. However, filament assembly in CHO and SV40-transformed lens-epithelial cells (both of which are fibroblast-like) yields radial networks which codistribute with the endogenous vimentin IFs. These observations document that the filaments formed by lens-specific IF proteins are structurally distinct from ordinary cytoplasmic IFs. Furthermore, the results suggest that the spatial arrangement of filensin/phakinin filaments in vivo is subject to regulation by host-specific factors. These factors may involve cytoskeletal networks (e.g., vimentin IFs) and/or specific sites associated with the cellular membranes.

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Year:  1996        PMID: 8647895      PMCID: PMC2199861          DOI: 10.1083/jcb.132.4.643

Source DB:  PubMed          Journal:  J Cell Biol        ISSN: 0021-9525            Impact factor:   10.539


  33 in total

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4.  Preparation of single molecules and supramolecular complexes for high-resolution metal shadowing.

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5.  Phosphorylation of chick lens proteins.

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8.  Visualization of a 21-nm axial periodicity in shadowed keratin filaments and neurofilaments.

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9.  The fibrillar substructure of keratin filaments unraveled.

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  16 in total

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3.  Autosomal recessive juvenile onset cataract associated with mutation in BFSP1.

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Review 4.  Functions of the intermediate filament cytoskeleton in the eye lens.

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Review 5.  Intermediate filaments as dynamic structures.

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Review 7.  Insights into the beaded filament of the eye lens.

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Review 8.  Development and application of STEM for the biological sciences.

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10.  Removal of Hsf4 leads to cataract development in mice through down-regulation of gamma S-crystallin and Bfsp expression.

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