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超顺磁性氧化铁纳米颗粒的巨噬细胞内吞作用:机制以及菲立磁和10-多聚麦芽糖铁的比较

Macrophage endocytosis of superparamagnetic iron oxide nanoparticles: mechanisms and comparison of ferumoxides and ferumoxtran-10.

作者信息

Raynal Isabelle, Prigent Philippe, Peyramaure Sophie, Najid Abderrahim, Rebuzzi Cécile, Corot Claire

机构信息

Guerbet-Research Department, Roissy CdG Cedex, France.

出版信息

Invest Radiol. 2004 Jan;39(1):56-63. doi: 10.1097/01.rli.0000101027.57021.28.

Abstract

RATIONALE AND OBJECTIVES

Superparamagnetic iron oxides (SPIO) used as magnetic resonance (MR) contrast agents undergo specific uptake by macrophages. The purpose of this study was first to determine the mechanism of macrophage uptake for Ferumoxides by using competition experiments with specific ligands of scavenger receptors SR-A (I/II) and second, to evaluate and compare the internalization of 2 different contrast agents, Ferumoxides (SPIO) and Ferumoxtran-10 (USPIO: ultrasmall superparamagnetic iron oxide) using macrophages obtained by chemical activation of human monocytic cells.

METHODS

Ferumoxides and Ferumoxtran-10 are 2 MR contrast agents, composed of dextran-coated iron oxide nanoparticles. The endocytosis pathway of Ferumoxides was studied using competition experiments on mouse peritoneal macrophages in the presence of specific ligands of scavenger receptors SR-A (types I and II): polyinosinic acid and fucoidan. In vitro assays using THP-1 (human promonocyte) cells activated into macrophages were performed in the presence of the 2 superparamagnetic nanoparticles. The cellular uptake was determined by measuring the iron content using ICP-AES (inductively coupled plasma-atomic emission spectrometry) and by Prussian blue staining.

RESULTS

In the presence of polyinosinic acid or fucoidan, the endocytosis of Ferumoxides by mouse peritoneal macrophages was inhibited. This inhibition was obtained using 10 microg/mL of scavenger receptor ligands at a concentration of 62.5 microg Fe/mL of SPIO, and a dose-dependent relationship was observed. Without competitors, the percentage of uptake of Ferumoxides by mouse peritoneal macrophages ranged between 3 and 8%. On the human activated monocyte THP-1 cell assay, Ferumoxides underwent a higher macrophage uptake (between 1.1 and 3%) compared with Ferumoxtran-10 (between 0.03 and 0.12%). This difference is attributed to the larger size of Ferumoxides nanoparticles.

CONCLUSIONS

Competition experiments indicate that the cellular uptake of Ferumoxides involves scavenger receptor SR-A-mediated endocytosis. The comparison between Ferumoxides and Ferumoxtran-10 confirms that macrophage uptake of iron oxide nanoparticles depends mainly on the size of these contrast agents.

摘要

原理与目的

用作磁共振(MR)造影剂的超顺磁性氧化铁(SPIO)会被巨噬细胞特异性摄取。本研究的目的首先是通过使用清道夫受体SR - A(I/II)的特异性配体进行竞争实验来确定巨噬细胞摄取菲立磁(Ferumoxides)的机制,其次是使用通过化学激活人单核细胞获得的巨噬细胞来评估和比较两种不同造影剂菲立磁(SPIO)和菲柔葡聚糖 - 10(USPIO:超小超顺磁性氧化铁)的内化情况。

方法

菲立磁和菲柔葡聚糖 - 10是两种MR造影剂,由葡聚糖包被的氧化铁纳米颗粒组成。在存在清道夫受体SR - A(I型和II型)的特异性配体:聚肌苷酸和岩藻依聚糖的情况下,通过对小鼠腹腔巨噬细胞进行竞争实验来研究菲立磁的内吞途径。在存在两种超顺磁性纳米颗粒的情况下,使用被激活为巨噬细胞的THP - 1(人原单核细胞)细胞进行体外测定。通过使用电感耦合等离子体原子发射光谱法(ICP - AES)测量铁含量以及普鲁士蓝染色来确定细胞摄取情况。

结果

在存在聚肌苷酸或岩藻依聚糖的情况下,小鼠腹腔巨噬细胞对菲立磁的内吞作用受到抑制。在菲立磁浓度为62.5μg Fe/mL时,使用10μg/mL的清道夫受体配体可获得这种抑制作用,并且观察到剂量依赖性关系。在没有竞争者的情况下,小鼠腹腔巨噬细胞对菲立磁的摄取百分比在3%至8%之间。在人激活的单核细胞THP - 1细胞测定中,与菲柔葡聚糖 - 10(在0.03%至0.12%之间)相比,菲立磁的巨噬细胞摄取率更高(在1.1%至3%之间)。这种差异归因于菲立磁纳米颗粒的尺寸更大。

结论

竞争实验表明,菲立磁的细胞摄取涉及清道夫受体SR - A介导的内吞作用。菲立磁和菲柔葡聚糖 - 10之间的比较证实,巨噬细胞对氧化铁纳米颗粒的摄取主要取决于这些造影剂的尺寸。

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