Thermostabilizing mutations in reovirus outer-capsid protein μ1 selected by heat inactivation of infectious subvirion particles

Jason K. Middleton; Melina A. Agosto; Tonya F. Severson; John Yin; Max L. Nibert

doi:10.1016/j.virol.2006.11.024

Thermostabilizing mutations in reovirus outer-capsid protein μ1 selected by heat inactivation of infectious subvirion particles

Jason K. Middleton, Melina A. Agosto, Tonya F. Severson, John Yin, Max L. Nibert

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Resumen

The 76-kDa μ1 protein of nonfusogenic mammalian reovirus is a major component of the virion outer capsid, which contains 200 μ1 trimers arranged in an incomplete T = 13 lattice. In virions, μ1 is largely covered by a second major outer-capsid protein, σ3, which limits μ1 conformational mobility. In infectious subvirion particles, from which σ3 has been removed, μ1 is broadly exposed on the surface and can be promoted to rearrange into a protease-sensitive and hydrophobic conformer, leading to membrane perforation or penetration. In this study, mutants that resisted loss of infectivity upon heat inactivation (heat-resistant mutants) were selected from infectious subvirion particles of reovirus strains Type 1 Lang and Type 3 Dearing. All of the mutants were found to have mutations in μ1, and the heat-resistance phenotype was mapped to μ1 by both recoating and reassortant genetics. Heat-resistant mutants were also resistant to rearrangement to the protease-sensitive conformer of μ1, suggesting that heat inactivation is associated with μ1 rearrangement, consistent with published results. Rate constants of heat inactivation were determined, and the dependence of inactivation rate on temperature was consistent with the Arrhenius relationship. The Gibbs free energy of activation was calculated with reference to transition-state theory and was found to be correlated with the degree of heat resistance in each of the analyzed mutants. The mutations are located in upper portions of the μ1 trimer, near intersubunit contacts either within or between trimers in the viral outer capsid. We propose that the mutants stabilize the outer capsid by interfering with unwinding of the μ1 trimer.

Idioma original	English
Páginas (desde-hasta)	412-425
Número de páginas	14
Publicación	Virology
Volumen	361
N.º	2
DOI	https://doi.org/10.1016/j.virol.2006.11.024
Estado	Published - may. 10 2007
Publicado de forma externa	Sí

Nota bibliográfica

Funding Information:
We are grateful to Laura Breun, Elaine Freimont, and Becky Margraf for technical assistance. We also thank Kartik Chandran, Steve Harrison, Tijana Ivanovic, and Lan Zhang for helpful comments on the manuscript. This study was supported in part by NIH grants F31AI064142 to M.A.A., R21 AI071197 to J.Y., and R01 AI46440 to M.L.N.; by NSF grant EIA-0331337 to J.Y.; and by a grant from the Lucille P. Markey Charitable Trust to the Institute for Molecular Virology at the University of Wisconsin-Madison. J.K.M. received support from The National Library of Medicine grant 5T15LM007359 as well as from NIH training grant T32 GM08349 to the Biotechnology program at the University of Wisconsin-Madison. M.A.A. received additional support from NIH training grant T32 GM07226 to the Biological and Biomedical Sciences program at Harvard University, Division of Medical Sciences.

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Virology

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title = "Thermostabilizing mutations in reovirus outer-capsid protein μ1 selected by heat inactivation of infectious subvirion particles",

abstract = "The 76-kDa μ1 protein of nonfusogenic mammalian reovirus is a major component of the virion outer capsid, which contains 200 μ1 trimers arranged in an incomplete T = 13 lattice. In virions, μ1 is largely covered by a second major outer-capsid protein, σ3, which limits μ1 conformational mobility. In infectious subvirion particles, from which σ3 has been removed, μ1 is broadly exposed on the surface and can be promoted to rearrange into a protease-sensitive and hydrophobic conformer, leading to membrane perforation or penetration. In this study, mutants that resisted loss of infectivity upon heat inactivation (heat-resistant mutants) were selected from infectious subvirion particles of reovirus strains Type 1 Lang and Type 3 Dearing. All of the mutants were found to have mutations in μ1, and the heat-resistance phenotype was mapped to μ1 by both recoating and reassortant genetics. Heat-resistant mutants were also resistant to rearrangement to the protease-sensitive conformer of μ1, suggesting that heat inactivation is associated with μ1 rearrangement, consistent with published results. Rate constants of heat inactivation were determined, and the dependence of inactivation rate on temperature was consistent with the Arrhenius relationship. The Gibbs free energy of activation was calculated with reference to transition-state theory and was found to be correlated with the degree of heat resistance in each of the analyzed mutants. The mutations are located in upper portions of the μ1 trimer, near intersubunit contacts either within or between trimers in the viral outer capsid. We propose that the mutants stabilize the outer capsid by interfering with unwinding of the μ1 trimer.",

author = "Middleton, {Jason K.} and Agosto, {Melina A.} and Severson, {Tonya F.} and John Yin and Nibert, {Max L.}",

note = "Funding Information: We are grateful to Laura Breun, Elaine Freimont, and Becky Margraf for technical assistance. We also thank Kartik Chandran, Steve Harrison, Tijana Ivanovic, and Lan Zhang for helpful comments on the manuscript. This study was supported in part by NIH grants F31AI064142 to M.A.A., R21 AI071197 to J.Y., and R01 AI46440 to M.L.N.; by NSF grant EIA-0331337 to J.Y.; and by a grant from the Lucille P. Markey Charitable Trust to the Institute for Molecular Virology at the University of Wisconsin-Madison. J.K.M. received support from The National Library of Medicine grant 5T15LM007359 as well as from NIH training grant T32 GM08349 to the Biotechnology program at the University of Wisconsin-Madison. M.A.A. received additional support from NIH training grant T32 GM07226 to the Biological and Biomedical Sciences program at Harvard University, Division of Medical Sciences. ",

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T1 - Thermostabilizing mutations in reovirus outer-capsid protein μ1 selected by heat inactivation of infectious subvirion particles

AU - Middleton, Jason K.

AU - Agosto, Melina A.

AU - Severson, Tonya F.

AU - Yin, John

AU - Nibert, Max L.

N1 - Funding Information: We are grateful to Laura Breun, Elaine Freimont, and Becky Margraf for technical assistance. We also thank Kartik Chandran, Steve Harrison, Tijana Ivanovic, and Lan Zhang for helpful comments on the manuscript. This study was supported in part by NIH grants F31AI064142 to M.A.A., R21 AI071197 to J.Y., and R01 AI46440 to M.L.N.; by NSF grant EIA-0331337 to J.Y.; and by a grant from the Lucille P. Markey Charitable Trust to the Institute for Molecular Virology at the University of Wisconsin-Madison. J.K.M. received support from The National Library of Medicine grant 5T15LM007359 as well as from NIH training grant T32 GM08349 to the Biotechnology program at the University of Wisconsin-Madison. M.A.A. received additional support from NIH training grant T32 GM07226 to the Biological and Biomedical Sciences program at Harvard University, Division of Medical Sciences.

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Y1 - 2007/5/10

N2 - The 76-kDa μ1 protein of nonfusogenic mammalian reovirus is a major component of the virion outer capsid, which contains 200 μ1 trimers arranged in an incomplete T = 13 lattice. In virions, μ1 is largely covered by a second major outer-capsid protein, σ3, which limits μ1 conformational mobility. In infectious subvirion particles, from which σ3 has been removed, μ1 is broadly exposed on the surface and can be promoted to rearrange into a protease-sensitive and hydrophobic conformer, leading to membrane perforation or penetration. In this study, mutants that resisted loss of infectivity upon heat inactivation (heat-resistant mutants) were selected from infectious subvirion particles of reovirus strains Type 1 Lang and Type 3 Dearing. All of the mutants were found to have mutations in μ1, and the heat-resistance phenotype was mapped to μ1 by both recoating and reassortant genetics. Heat-resistant mutants were also resistant to rearrangement to the protease-sensitive conformer of μ1, suggesting that heat inactivation is associated with μ1 rearrangement, consistent with published results. Rate constants of heat inactivation were determined, and the dependence of inactivation rate on temperature was consistent with the Arrhenius relationship. The Gibbs free energy of activation was calculated with reference to transition-state theory and was found to be correlated with the degree of heat resistance in each of the analyzed mutants. The mutations are located in upper portions of the μ1 trimer, near intersubunit contacts either within or between trimers in the viral outer capsid. We propose that the mutants stabilize the outer capsid by interfering with unwinding of the μ1 trimer.

AB - The 76-kDa μ1 protein of nonfusogenic mammalian reovirus is a major component of the virion outer capsid, which contains 200 μ1 trimers arranged in an incomplete T = 13 lattice. In virions, μ1 is largely covered by a second major outer-capsid protein, σ3, which limits μ1 conformational mobility. In infectious subvirion particles, from which σ3 has been removed, μ1 is broadly exposed on the surface and can be promoted to rearrange into a protease-sensitive and hydrophobic conformer, leading to membrane perforation or penetration. In this study, mutants that resisted loss of infectivity upon heat inactivation (heat-resistant mutants) were selected from infectious subvirion particles of reovirus strains Type 1 Lang and Type 3 Dearing. All of the mutants were found to have mutations in μ1, and the heat-resistance phenotype was mapped to μ1 by both recoating and reassortant genetics. Heat-resistant mutants were also resistant to rearrangement to the protease-sensitive conformer of μ1, suggesting that heat inactivation is associated with μ1 rearrangement, consistent with published results. Rate constants of heat inactivation were determined, and the dependence of inactivation rate on temperature was consistent with the Arrhenius relationship. The Gibbs free energy of activation was calculated with reference to transition-state theory and was found to be correlated with the degree of heat resistance in each of the analyzed mutants. The mutations are located in upper portions of the μ1 trimer, near intersubunit contacts either within or between trimers in the viral outer capsid. We propose that the mutants stabilize the outer capsid by interfering with unwinding of the μ1 trimer.

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Thermostabilizing mutations in reovirus outer-capsid protein μ1 selected by heat inactivation of infectious subvirion particles

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