Literature DB >> 23903836

The respiratory syncytial virus fusion protein targets to the perimeter of inclusion bodies and facilitates filament formation by a cytoplasmic tail-dependent mechanism.

Pradyumna S Baviskar1, Anne L Hotard, Martin L Moore, Antonius G P Oomens.   

Abstract

The human respiratory syncytial virus (HRSV) fusion (F) protein cytoplasmic tail (CT) and matrix (M) protein are key mediators of viral assembly, but the underlying mechanisms are poorly understood. A complementation assay was developed to systematically examine the role of the F protein CT in infectious virus production. The ability of F mutants with alanine substitutions in the CT to complement an F-null virus in generating infectious progeny was quantitated by flow cytometry. Two CT regions with impact on infectious progeny production were identified: residues 557 to 566 (CT-R1) and 569 to 572 (CT-R2). Substitutions in CT-R1 decreased infectivity by 40 to 85% and increased the level of F-induced cell-cell fusion but had little impact on assembly of viral surface filaments, which are believed to be virions. Substitutions in CT-R2, as well as deletion of the entire CT, abrogated infectious progeny production and impaired viral filament formation. However, CT-R2 mutations did not block but rather delayed the formation of viral filaments, which continued to form at a low rate and contained the viral M protein and nucleoprotein (N). Microscopy analysis revealed that substitutions in CT-R2 but not CT-R1 led to accumulation of M and F proteins within and at the perimeter of viral inclusion bodies (IBs), respectively. The accumulation of M and F at IBs and coincident strong decrease in filament formation and infectivity upon CT-R2 mutations suggest that F interaction with IBs is an important step in the virion assembly process and that CT residues 569 to 572 act to facilitate release of M-ribonucleoprotein complexes from IBs.

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Year:  2013        PMID: 23903836      PMCID: PMC3807408          DOI: 10.1128/JVI.03086-12

Source DB:  PubMed          Journal:  J Virol        ISSN: 0022-538X            Impact factor:   5.103


  49 in total

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4.  Association of respiratory syncytial virus M protein with viral nucleocapsids is mediated by the M2-1 protein.

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5.  Human respiratory syncytial virus nucleoprotein and inclusion bodies antagonize the innate immune response mediated by MDA5 and MAVS.

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7.  Influence of lipids on the interfacial disposition of respiratory syncytical virus matrix protein.

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10.  Sorting of the respiratory syncytial virus matrix protein into detergent-resistant structures is dependent on cell-surface expression of the glycoproteins.

Authors:  Gary Henderson; Jillian Murray; Robert P Yeo
Journal:  Virology       Date:  2002-09-01       Impact factor: 3.616

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3.  The Thr205 phosphorylation site within respiratory syncytial virus matrix (M) protein modulates M oligomerization and virus production.

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4.  Identification of residues in the human respiratory syncytial virus fusion protein that modulate fusion activity and pathogenesis.

Authors:  Anne L Hotard; Sujin Lee; Michael G Currier; James E Crowe; Kaori Sakamoto; Dawn C Newcomb; R Stokes Peebles; Richard K Plemper; Martin L Moore
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5.  New host factors important for respiratory syncytial virus (RSV) replication revealed by a novel microfluidics screen for interactors of matrix (M) protein.

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Journal:  Mol Cell Proteomics       Date:  2015-01-02       Impact factor: 5.911

6.  Dimerization of matrix protein is required for budding of respiratory syncytial virus.

Authors:  Andreas Förster; Goedele N Maertens; Paul J Farrell; Monika Bajorek
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7.  Adaptor complex-mediated trafficking of Newcastle disease virus fusion protein is regulated by the YLMY motif of its cytoplasmic tail.

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9.  Functional correlations of respiratory syncytial virus proteins to intrinsic disorder.

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Review 10.  Paramyxovirus glycoprotein incorporation, assembly and budding: a three way dance for infectious particle production.

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