4.6 Article

Multiprotein Adsorption from Human Serum at Gold and Oxidized Iron Surfaces Studied by Atomic Force Microscopy and Polarization-Modulation Infrared Reflection Absorption Spectroscopy

Journal

MOLECULES
Volume 28, Issue 16, Pages -

Publisher

MDPI
DOI: 10.3390/molecules28166060

Keywords

biointerfaces; protein adsorption; serum; AFM; PM-IRRAS

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This study investigates the multiprotein adsorption from diluted human serum at gold and oxidized iron surfaces, revealing stronger protein adsorption at pH 6. The changes in surface topography and the total amount of adsorbed proteins are quantified by atomic force microscopy and polarization-modulation infrared reflection absorption spectroscopy. Qualitative insights into the pH-dependent alterations in the composition of the adsorbed multiprotein films are provided by PM-IRRAS, suggesting a change in protein film composition at pH 6 accompanied by increased adsorption.
Multiprotein adsorption from complex body fluids represents a highly important and complicated phenomenon in medicine. In this work, multiprotein adsorption from diluted human serum at gold and oxidized iron surfaces is investigated at different serum concentrations and pH values. Adsorption-induced changes in surface topography and the total amount of adsorbed proteins are quantified by atomic force microscopy (AFM) and polarization-modulation infrared reflection absorption spectroscopy (PM-IRRAS), respectively. For both surfaces, stronger protein adsorption is observed at pH 6 compared to pH 7 and pH 8. PM-IRRAS furthermore provides some qualitative insights into the pH-dependent alterations in the composition of the adsorbed multiprotein films. Changes in the amide II/amide I band area ratio and in particular side-chain IR absorption suggest that the increased adsorption at pH 6 is accompanied by a change in protein film composition. Presumably, this is mostly driven by the adsorption of human serum albumin, which at pH 6 adsorbs more readily and thereby replaces other proteins with lower surface affinities in the resulting multiprotein film.

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