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Spectral demonstration of structural transitions in albumins. / Tankovskaia, Svetlana A.; Abrosimova, Karina V.; Paston, Sofia V.
в: Journal of Molecular Structure, Том 1171, 05.11.2018, стр. 243-252.Результаты исследований: Научные публикации в периодических изданиях › статья › Рецензирование
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TY - JOUR
T1 - Spectral demonstration of structural transitions in albumins
AU - Tankovskaia, Svetlana A.
AU - Abrosimova, Karina V.
AU - Paston, Sofia V.
PY - 2018/11/5
Y1 - 2018/11/5
N2 - Several spectral methods (UV absorbance, fluorescent and FTIR spectroscopy) were applied to reveal the alterations in the secondary and tertiary structures of human serum albumin (HSA) in water solutions under various conditions (pH, protein concentration, ethanol and n-propanol addition). The structural transitions well known for defatted HSA at 1.5 < pH < 13 are observed for HSA in a complex with long-chain fatty acids in the molar ratio about 1:1. The changes of HSA ζ-potential during the protein isomerizations induced by the variation of pH are traced. It is shown that HSA does not completely lose its secondary structure at extreme alkaline or acidic solutions, which indicates that at these conditions HSA takes the “molten globule” conformation. A comparison of aggregation processes of HSA and ovalbumin in neutral water and 0.15 M NaCl solutions reveals that OVA aggregation is preceded by a partially denaturated state of the protein, whereas an intermediates of HSA aggregates are close to the native state of the protein. The aliphatic alcohols disturb the tertiary structure of HSA, but stabilize its secondary structure. This effect increases with the rise of the alcohol hydrophobicity.
AB - Several spectral methods (UV absorbance, fluorescent and FTIR spectroscopy) were applied to reveal the alterations in the secondary and tertiary structures of human serum albumin (HSA) in water solutions under various conditions (pH, protein concentration, ethanol and n-propanol addition). The structural transitions well known for defatted HSA at 1.5 < pH < 13 are observed for HSA in a complex with long-chain fatty acids in the molar ratio about 1:1. The changes of HSA ζ-potential during the protein isomerizations induced by the variation of pH are traced. It is shown that HSA does not completely lose its secondary structure at extreme alkaline or acidic solutions, which indicates that at these conditions HSA takes the “molten globule” conformation. A comparison of aggregation processes of HSA and ovalbumin in neutral water and 0.15 M NaCl solutions reveals that OVA aggregation is preceded by a partially denaturated state of the protein, whereas an intermediates of HSA aggregates are close to the native state of the protein. The aliphatic alcohols disturb the tertiary structure of HSA, but stabilize its secondary structure. This effect increases with the rise of the alcohol hydrophobicity.
KW - Aliphatic alcohols
KW - FTIR spectroscopy
KW - Intrinsic protein fluorescence
KW - Ovalbumin
KW - Secondary and tertiary structure of protein
KW - Serum albumin
KW - UV absorbance spectroscopy
UR - http://www.scopus.com/inward/record.url?scp=85048300843&partnerID=8YFLogxK
U2 - 10.1016/j.molstruc.2018.05.100
DO - 10.1016/j.molstruc.2018.05.100
M3 - Article
AN - SCOPUS:85048300843
VL - 1171
SP - 243
EP - 252
JO - Journal of Molecular Structure
JF - Journal of Molecular Structure
SN - 0022-2860
ER -
ID: 41697771