Comparing qualitative and quantitative spectroscopic techniques for the detection of the effect of direct iron loading of mammalian cell cultures.

H N Traore, D Meyer
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引用次数: 10

Abstract

Iron overload augments diseases of the liver and microorganism infection as well as deregulates the immune system. In vitro analysis of the effects of iron loading and its chelation involves determining the amount of iron constituting overload, which metal sources and cell lines to use and reliable assay methods. The uptake of 500 microM FeSO4 or FeEDTA by CEMss, U937 or leukocytes was confirmed by inductively coupled plasma-atomic emission spectroscopy (ICP-AES). Excess iron increased CEMss viability (assessed by MTT, XTT, Trypan- and Alamar Blue) by an average of 18% (P = 0.034). Flow cytometry indicated dye-viable cells to be undergoing apotosis/necrosis while still confirming an increase (9%, P < 0.001) in excess iron-induced viability. The iron chelator desferioxamine (DFO) when added in addition to Fe, reversed the effects of excess iron (and vice versa) and had detrimental effects when used on its own (33% inhibition of viability as measured by dyes and 10.85%; P = 0.0427 assessed by flow cytometry). The 4 dyes demonstrated different levels of sensitivity in detecting the influence of iron or DFO but gave a related, qualitative picture while flow cytometry and ICP-AES data was more quantitative.

比较定性和定量光谱技术对哺乳动物细胞培养物直接铁负载效果的检测。
铁超载会增加肝脏疾病和微生物感染,并使免疫系统失调。铁负载及其螯合作用的体外分析包括确定铁的过载量,使用哪种金属来源和细胞系以及可靠的测定方法。通过电感耦合等离子体原子发射光谱(ICP-AES)证实了cems、U937或白细胞对500微米FeSO4或FeEDTA的摄取。过量的铁使CEMss活力(MTT、XTT、Trypan-和Alamar Blue评估)平均提高18% (P = 0.034)。流式细胞术显示染料活细胞正在发生凋亡/坏死,同时仍证实过量铁诱导的活力增加(9%,P < 0.001)。铁螯合剂去铁胺(DFO)在加入铁的同时,可以逆转过量铁的影响(反之亦然),但单独使用时却有不利影响(染料测定的活力抑制率为33%,10.85%;流式细胞术P = 0.0427)。4种染料在检测铁或DFO的影响时表现出不同程度的敏感性,但给出了相关的定性图像,而流式细胞术和ICP-AES数据更为定量。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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