Development of a fast and simple method for the isolation of superparamagnetic iron oxide nanoparticles protein corona from protein-rich matrices

离心 超顺磁性 化学 生物分子 日冕(行星地质学) 分离(微生物学) 纳米颗粒 吸附 差速离心 色谱法 磁性纳米粒子 蛋白质吸附 生物物理学 纳米技术 材料科学 生物化学 生物 生物信息学 有机化学 物理 磁化 量子力学 天体生物学 磁场 维纳斯
作者
Mahmoud G. Soliman,Duong N. Trinh,Costanza Ravagli,Paula Meleady,Michael Henry,Dania Movia,Saer Doumett,Laura Cappiello,Adriele Prina‐Mello,Giovanni Baldi,Marco P. Monopoli
出处
期刊:Journal of Colloid and Interface Science [Elsevier BV]
卷期号:659: 503-519 被引量:9
标识
DOI:10.1016/j.jcis.2023.11.177
摘要

The adsorption of proteins onto the surface of nanoparticle (NP) leads to the formation of the so-called "protein corona" as consisting both loosely and tightly bound proteins. It is well established that the biological identity of NPs that may be acquired after exposure to a biological matrix is mostly provided by the components of the hard corona as the pristine surface is generally less accessible for binding. For that reason, the isolation and the characterisation of the NP-corona complexes and identification of the associated biomolecules can help in understanding its biological behaviour. Established methods for the isolation of the NP-HC complexes are time-demanding and can lead to different results based on the isolation method applied. Herein, we have developed a fast and simple method using ferromagnetic beads isolated from commercial MACS column and used for the isolation of superparamagnetic NP following exposure to different types of biological milieu. We first demonstrated the ability to easily isolate superparamagnetic iron oxide NPs (IONPs) from different concentrations of human blood plasma, and also tested the method on the corona isolation using more complex biological matrices, such as culture medium containing pulmonary mucus where the ordinary corona methods cannot be applied. Our developed method showed less than 20% difference in plasma corona composition when compared with centrifugation. It also showed effective isolation of NP-HC complexes from mucus-containing culture media upon comparing with centrifugation and MACS columns, which failed to wash out the unbound proteins. Our study was supported with a full characterisation profile including dynamic light scattering, nanoparticle tracking analysis, analytical disk centrifuge, and zeta potentials. The biomolecules/ proteins composing the HC were separated by vertical gel electrophoresis and subsequently analysed by liquid chromatography-tandem mass spectrometry. In addition to our achievements in comparing different isolation methods to separate IONPs with corona from human plasma, this is the first study that provides a complete characterisation profile of particle protein corona after exposure in vitro to pulmonary mucus-containing culture media.
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