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铁蛋白铁的还原性释放:一种动力学测定法。

Reductive release of ferritin iron: a kinetic assay.

作者信息

Boyer R F, Grabill T W, Petrovich R M

机构信息

Department of Chemistry, Hope College, Holland, Michigan 49423.

出版信息

Anal Biochem. 1988 Oct;174(1):17-22. doi: 10.1016/0003-2697(88)90513-1.

Abstract

Ferritin iron release, a process of considerable interest in biology and medicine, occurs most readily in the presence of reducing agents. Here is described a kinetic assay for measuring the rate of ferritin iron removal promoted by various reductants. The new procedure uses ferrozine as a chromophoric, high-affinity chelator for the product, Fe(II). The initial rate of iron release is quantified by continuous spectrophotometric measurement of the Fe(ferrozine)2/3+ complex which absorbs maximally at 562 nm. The initial rate of iron mobilization is dependent on reductant concentration, but not on the concentration of the chelating agent, ferrozine. Saturation kinetics are observed for all reductants, including dihydroxyfumarate, cysteine, caffeic acid, ascorbate, and glutathione. Superoxide dismutase greatly inhibits ferritin iron release by ascorbate, but has little or no effect on the reducing action of dihydroxyfumarate, cysteine, caffeic acid, or glutathione. Ferritin iron removal by dihydroxyfumarate was inhibited by various metal ions. This new assay may be used for rapid screening of test compounds for treatment of iron overload and for investigation of the mechanistic aspects of ferritin iron reduction.

摘要

铁蛋白铁释放是生物学和医学中一个备受关注的过程,在还原剂存在的情况下最容易发生。本文描述了一种动力学测定方法,用于测量各种还原剂促进铁蛋白铁去除的速率。新方法使用亚铁嗪作为产物Fe(II)的发色高亲和力螯合剂。通过连续分光光度法测量在562 nm处有最大吸收的Fe(亚铁嗪)2/3+络合物来定量铁释放的初始速率。铁动员的初始速率取决于还原剂浓度,但不取决于螯合剂亚铁嗪的浓度。对所有还原剂,包括二羟基富马酸、半胱氨酸、咖啡酸、抗坏血酸和谷胱甘肽,均观察到饱和动力学。超氧化物歧化酶极大地抑制了抗坏血酸引起的铁蛋白铁释放,但对二羟基富马酸、半胱氨酸、咖啡酸或谷胱甘肽的还原作用几乎没有影响。二羟基富马酸去除铁蛋白铁的过程受到各种金属离子的抑制。这种新的测定方法可用于快速筛选治疗铁过载的测试化合物,以及研究铁蛋白铁还原的机制方面。

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