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Effect of dietary iron deficiency and overload on the expression of ZIP metal-ion transporters in rat liver

机译:饮食中铁缺乏和超负荷对大鼠肝脏ZIP金属离子转运蛋白表达的影响

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The mammalian ZIP (Zrt-, Irt-like Protein) family of transmembrane transport proteins consists of 14 members that share considerable homology. ZIP proteins have been shown to mediate the cellular uptake of the essential trace elements zinc, iron, and manganese. The aim of the present study was to determine the effect of dietary iron deficiency and overload on the expression of all 14 ZIP transporters in the liver, the main site of iron storage. Weanling male rats (n = 6/group) were fed iron-deficient (FeD), iron-adequate (FeA), or iron-overloaded (FeO) diets in two independent feeding studies. In study 1, diets were based on the TestDiet 5755 formulation and contained iron at 9 ppm (FeD), 215 ppm (FeA), and 27,974 ppm (3% FeO). In study 2, diets were based on the AIN-93G formulation and contained iron at 9 ppm Fe (FeD), 50 ppm Fe (FeA), or 18916 ppm (2% FeO). After 3 weeks, the FeD diets depleted liver non-heme iron stores and induced anemia, whereas FeO diets resulted in hepatic iron overload. Quantitative RT-PCR revealed that ZIP5 mRNA levels were 3- and 8-fold higher in 2% FeO and 3% FeO livers, respectively, compared with FeA controls. In both studies, a consistent downregulation of ZIP6, ZIP7, and ZIP10 was also observed in FeO liver relative to FeA controls. Studies in H4IIE hepatoma cells further documented that iron loading affects the expression of these ZIP transporters. Overall, our data suggest that ZIP5, ZIP6, ZIP7, and ZIP10 are regulated by iron, indicating that they may play a role in hepatic iron/metal homeostasis during iron deficiency and overload.
机译:跨膜转运蛋白的哺乳动物ZIP(Zrt-,Irt-like蛋白)家族由14个成员组成,它们具有相当的同源性。已显示ZIP蛋白可介导细胞摄取必需的微量元素锌,铁和锰。本研究的目的是确定饮食中铁缺乏和铁过量对所有14种ZIP转运蛋白在肝脏中的表达的影响,肝脏是铁储存的主要部位。在两项独立的喂养研究中,对断奶的雄性大鼠(n = 6 /组)饲喂缺铁(FeD),充足铁(FeA)或过量铁(FeO)饮食。在研究1中,饮食以TestDiet 5755配方为基础,并且铁含量分别为9 ppm(FeD),215 ppm(FeA)和27,974 ppm(3%FeO)。在研究2中,饮食基于AIN-93G配方,并含有9 ppm Fe(FeD),50 ppm Fe(FeA)或18916 ppm(2%FeO)的铁。 3周后,FeD饮食耗尽了肝脏的非血红素铁储备并引发了贫血,而FeO饮食则导致肝铁超负荷。定量RT-PCR显示,与FeA对照相比,在2%FeO和3%FeO肝脏中ZIP5 mRNA水平分别高3倍和8倍。在两项研究中,相对于FeA对照,在FeO肝脏中还观察到ZIP6,ZIP7和ZIP10的一致下调。对H4IIE肝癌细胞的研究进一步证明,铁负载会影响这些ZIP转运蛋白的表达。总体而言,我们的数据表明ZIP5,ZIP6,ZIP7和ZIP10受铁的调节,表明它们可能在铁缺乏和超负荷时在肝铁/金属稳态中起作用。

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