Heat-Denatured Lysozyme Aggregation and Gelation As Revealed by Combined Dielectric Relaxation Spectroscopy and Light Scattering Measurements

The dielectric behavior of native and heat-denatured lysozyme in ethanol–water solutions was examined in the frequency range from 1 MHz to 2 GHz, using frequency-domain dielectric relaxation spectroscopy. Because of the conformational changes on unfolding, dielectric methods provide information on t...

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Veröffentlicht in:	The journal of physical chemistry. B 2012-09, Vol.116 (35), p.10779-10785
Hauptverfasser:	Giugliarelli, A, Sassi, P, Paolantoni, M, Onori, G, Cametti, C
Format:	Artikel
Sprache:	eng
Schlagworte:	Agglomeration Denaturation Dielectric relaxation Dielectric Spectroscopy Ethanol - chemistry Gelation Gels - chemistry Light Light scattering Lysozyme Muramidase - chemistry Muramidase - metabolism Polystyrenes - chemistry Protein Denaturation Proteins Scattering, Radiation Spectroscopy Temperature Water - chemistry
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container_end_page	10785
container_issue	35
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container_title	The journal of physical chemistry. B
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creator	Giugliarelli, A Sassi, P Paolantoni, M Onori, G Cametti, C
description	The dielectric behavior of native and heat-denatured lysozyme in ethanol–water solutions was examined in the frequency range from 1 MHz to 2 GHz, using frequency-domain dielectric relaxation spectroscopy. Because of the conformational changes on unfolding, dielectric methods provide information on the denaturation process of the protein and, at protein concentration high enough, on the subsequent aggregation and gelation. Moreover, the time evolution of the protein aggregation and gelation was monitored measuring, by means of dynamic light scattering methods, the diffusion coefficient of micro-sized polystyrene particles, deliberately added to the protein solution, which act as a probe of the viscosity of the microenvironment close to the particle surface. All together, our measurements indicate that heat-induced denaturation favors, at high concentrations, a protein aggregation process which evolves up to the full gelation of the system. These findings have a direct support from IR measurements of the absorbance of the amide I band that, because of the unfolding, indicate that proteins entangle each other, producing a network structure which evolves, in long time limit, in the gel.
doi_str_mv	10.1021/jp305939h
format	Article
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All together, our measurements indicate that heat-induced denaturation favors, at high concentrations, a protein aggregation process which evolves up to the full gelation of the system. 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B</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Giugliarelli, A</au><au>Sassi, P</au><au>Paolantoni, M</au><au>Onori, G</au><au>Cametti, C</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Heat-Denatured Lysozyme Aggregation and Gelation As Revealed by Combined Dielectric Relaxation Spectroscopy and Light Scattering Measurements</atitle><jtitle>The journal of physical chemistry. B</jtitle><addtitle>J. Phys. Chem. B</addtitle><date>2012-09-06</date><risdate>2012</risdate><volume>116</volume><issue>35</issue><spage>10779</spage><epage>10785</epage><pages>10779-10785</pages><issn>1520-6106</issn><eissn>1520-5207</eissn><abstract>The dielectric behavior of native and heat-denatured lysozyme in ethanol–water solutions was examined in the frequency range from 1 MHz to 2 GHz, using frequency-domain dielectric relaxation spectroscopy. Because of the conformational changes on unfolding, dielectric methods provide information on the denaturation process of the protein and, at protein concentration high enough, on the subsequent aggregation and gelation. Moreover, the time evolution of the protein aggregation and gelation was monitored measuring, by means of dynamic light scattering methods, the diffusion coefficient of micro-sized polystyrene particles, deliberately added to the protein solution, which act as a probe of the viscosity of the microenvironment close to the particle surface. All together, our measurements indicate that heat-induced denaturation favors, at high concentrations, a protein aggregation process which evolves up to the full gelation of the system. These findings have a direct support from IR measurements of the absorbance of the amide I band that, because of the unfolding, indicate that proteins entangle each other, producing a network structure which evolves, in long time limit, in the gel.</abstract><cop>United States</cop><pub>American Chemical Society</pub><pmid>22891653</pmid><doi>10.1021/jp305939h</doi><tpages>7</tpages></addata></record>
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subjects	Agglomeration Denaturation Dielectric relaxation Dielectric Spectroscopy Ethanol - chemistry Gelation Gels - chemistry Light Light scattering Lysozyme Muramidase - chemistry Muramidase - metabolism Polystyrenes - chemistry Protein Denaturation Proteins Scattering, Radiation Spectroscopy Temperature Water - chemistry
title	Heat-Denatured Lysozyme Aggregation and Gelation As Revealed by Combined Dielectric Relaxation Spectroscopy and Light Scattering Measurements
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