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磁铁矿纳米颗粒的蛋白质外壳和纳米颗粒-蛋白质复合物被内吞进入健康细胞和癌细胞。

Protein corona on magnetite nanoparticles and internalization of nanoparticle-protein complexes into healthy and cancer cells.

机构信息

National Engineering Research Center for Biomaterials, Sichuan University, Chengdu, 610064, Sichuan, China.

出版信息

Arch Pharm Res. 2014 Jan;37(1):129-41. doi: 10.1007/s12272-013-0292-2. Epub 2013 Dec 6.

DOI:10.1007/s12272-013-0292-2
PMID:24310098
Abstract

Superparamagnetic magnetite nanoparticles (MNPs) of different surface properties are incubated in complicated living fluid, including fetal bovine serum solution, cell complete culture medium and cell culture system with/without serum, to investigate the alteration of protein corona and its impact on cell internalization. The MNPs prepared by co-precipitation method are functionalized with L-Lysine (Lys), Glucosamic acid (GA) to obtain amine, carboxyl and hydroxyl groups, separately. All the particles adsorb serum proteins to form MNPs-protein complexes with the surface charge changing into negative. 1D SDS/PAGE gel images analysis indicates that the composition and content of hard protein corona on the surface of NPs are related to their functional groups and agglomeration, and the total amount of protein in the medium. In cell culture system, particles not only adsorb serum proteins, but also associate with cytosolic proteins arising from HepG2 and L02 cells. GA modified MNPs (MNPs-GA) exhibit bovine serum albumin anti-adsorption capability because of the terminal hydroxyl and carboxyl groups. MNPs-GA also shows the highest cellular uptake and label efficiency compared with uncoated MNPs and Lys modified MNPs, due to larger aggregates formation and specific protein corona composition, rather than commonly approved electrostatic interaction between particles and cells. For the first time, our results provide visualized reports on previously neglected, but indispensable protein corona of the MNPs after interaction with both healthy and cancer cells, suggesting that cytosolic protein corona from cells and aggregation of particles are important factors needed to be account for on studying the nano-bio interface.

摘要

不同表面性质的超顺磁磁铁矿纳米颗粒(MNPs)在复杂的活体流体中孵育,包括胎牛血清溶液、细胞完全培养基以及有/无血清的细胞培养系统,以研究蛋白质冠的变化及其对细胞内化的影响。共沉淀法制备的 MNPs 通过 L-赖氨酸(Lys)、氨基葡萄糖酸(GA)进行功能化,分别获得氨基、羧基和羟基。所有颗粒都吸附血清蛋白,形成表面电荷变为负电荷的 MNPs-蛋白复合物。1D SDS/PAGE 凝胶图像分析表明,NP 表面硬蛋白冠的组成和含量与它们的官能团和聚集状态以及培养基中的总蛋白含量有关。在细胞培养系统中,颗粒不仅吸附血清蛋白,还与来自 HepG2 和 L02 细胞的胞质蛋白结合。由于末端的羟基和羧基,GA 修饰的 MNPs(MNPs-GA)表现出牛血清白蛋白抗吸附能力。与未涂层 MNPs 和 Lys 修饰的 MNPs 相比,MNPs-GA 还表现出更高的细胞摄取率和标记效率,这是由于更大的聚集形成和特定的蛋白冠组成,而不是颗粒和细胞之间通常认可的静电相互作用。我们的研究结果首次提供了关于 MNPs 与健康细胞和癌细胞相互作用后被忽视但不可或缺的蛋白冠的可视化报告,表明来自细胞的胞质蛋白冠和颗粒的聚集是在研究纳米生物界面时需要考虑的重要因素。

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