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Physical and Biological Characterization of Superparamagnetic Iron Oxide- and Ultrasmall Superparamagnetic Iron Oxide-Labeled Cells: A Comparison.

机译:超顺磁性氧化铁和超小型超顺磁性氧化铁标记细胞的物理和生物学特性:比较。

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RATIONALE:: Superparamagnetic iron-oxide particles are used frequently for cellular magnetic resonance imaging and in vivo cell tracking. The purpose of this study was to compare the labeling characteristics and efficiency as well as toxicity of superparamagnetic iron oxide (SPIO) and ultrasmall superparamagnetic iron oxide (USPIO) for 3 cell lines. METHODS:: Using human fibroblasts, immortalized rat progenitor cells and HEP-G2-hepatoma cells, dose- and time-dependence of SPIO and USPIO uptake were evaluated. The amount of intracellular (U)SPIO was monitored over 2 weeks after incubation by T2-magnetic resonance relaxometry, ICP-mass-spectrometry, and histology. Transmission-electronmicroscopy was used to specify the intracellular localization of the endocytosed iron particles. Cell death-rate and proliferation-index were assessed as indicators of cell-toxicity. RESULT:: For all cell lines, SPIO showed better uptake than USPIO, which was highest in HEP-G2 cells (110 +/- 2 pg Fe/cell). Cellular iron concentrations in progenitor cells and fibroblasts were 13 +/- 1pg Fe/cell and 7.2 +/- 0.3pg Fe/cell, respectively. For all cell lines T2-relaxation times in cell pellets were below detection threshold (<3 milliseconds) after 5 hours of incubation with SPIO (3.0 mumol Fe/mL growth medium) and continued to be near the detection for the next 6 days. For both particle types and all cell lines cellular iron oxide contents decreased after recultivation and surprisingly were found lower than in unlabeled control cells after 15 days. Viability and proliferation of (U)SPIO-labeled and unlabeled cells were not significantly different. CONCLUSIONS:: The hematopoetic progenitor, mesenchymal fibroblast and epithelial HEP-G2 cell lines accumulated SPIO more efficiently than USPIO indicating SPIO to be better suited for cell labeling. However, the results indicate that there may be an induction of forced cellular iron elimination after incubation with (U)SPIO.
机译:理由:超顺磁性氧化铁颗粒经常用于细胞磁共振成像和体内细胞追踪。本研究的目的是比较3种细胞系的超顺磁性氧化铁(SPIO)和超小型超顺磁性氧化铁(USPIO)的标记特性,效率以及毒性。方法:使用人类成纤维细胞,永生化的大鼠祖细胞和HEP-G2-肝癌细胞,评估SPIO和USPIO摄取的剂量和时间依赖性。孵育后2周内,通过T2磁共振弛豫法,ICP-质谱和组织学方法监测细胞内(U)SPIO的量。透射电镜用于确定胞吞铁颗粒的胞内定位。将细胞死亡率和增殖指数评估为细胞毒性的指标。结果:在所有细胞系中,SPIO的吸收均优于USPIO,这在HEP-G2细胞中最高(110 +/- 2 pg Fe /细胞)。祖细胞和成纤维细胞中的细胞铁浓度分别为13 +/- 1pg Fe /细胞和7.2 +/- 0.3pg Fe /细胞。对于所有细胞系,在与SPIO(3.0μmolFe / mL生长培养基)孵育5小时后,细胞沉淀中T2松弛时间低于检测阈值(<3毫秒),并且在接下来的6天中继续接近检测值。对于两种类型的颗粒和所有细胞系,细胞中的氧化铁含量在培养后都会降低,出人意料的是,在15天后发现其含量低于未标记的对照细胞。 (U)SPIO标记和未标记的细胞的活力和增殖没有显着差异。结论:造血祖细胞,间充质成纤维细胞和上皮性HEP-G2细胞系比USPIO更有效地积累SPIO,表明SPIO更适合细胞标记。但是,结果表明与(U)SPIO孵育后,可能会诱导强制性细胞铁清除。

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