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Nramp2铁转运蛋白在肠道刷状缘的细胞及亚细胞定位与膳食铁的调节作用

Cellular and subcellular localization of the Nramp2 iron transporter in the intestinal brush border and regulation by dietary iron.

作者信息

Canonne-Hergaux F, Gruenheid S, Ponka P, Gros P

机构信息

Departments of Biochemistry and Physiology, McGill University, Montreal, Quebec, Canada.

出版信息

Blood. 1999 Jun 15;93(12):4406-17.


DOI:
PMID:10361139
Abstract

Genetic studies in animal models of microcytic anemia and biochemical studies of transport have implicated the Nramp2 gene in iron transport. Nramp2 generates two alternatively spliced mRNAs that differ at their 3' untranslated region by the presence or absence of an iron-response element (IRE) and that encode two proteins with distinct carboxy termini. Antisera raised against Nramp2 fusion proteins containing either the carboxy or amino termini of Nramp2 and that can help distinguish between the two Nramp2 protein isoforms (IRE: isoform I; non-IRE: isoform II) were generated. These antibodies were used to identify the cellular and subcellular localization of Nramp2 in normal tissues and to study possible regulation by dietary iron deprivation. Immunoblotting experiments with membrane fractions from intact organs show that Nramp2 is expressed at low levels throughout the small intestine and to a higher extent in kidney. Dietary iron starvation results in a dramatic upregulation of the Nramp2 isoform I in the proximal portion of the duodenum only, whereas expression in the rest of the small intestine and in kidney remains largely unchanged in response to the lack of dietary iron. In proximal duodenum, immunostaining studies of tissue sections show that Nramp2 protein expression is abundant under iron deplete condition and limited to the villi and is absent in the crypts. In the villi, staining is limited to the columnar absorptive epithelium of the mucosa (enterocytes), with no expression in mucus-secreting goblet cells or in the lamina propria. Nramp2 expression is strongest in the apical two thirds of the villi and is very intense at the brush border of the apical pole of the enterocytes, whereas the basolateral membrane of these cells is negative for Nramp2. These results strongly suggest that Nramp2 is indeed responsible for transferrin-independent iron uptake in the duodenum. These findings are discussed in the context of overall mechanisms of iron acquisition by the body.

摘要

在小细胞贫血动物模型中的遗传学研究以及转运的生化研究表明,Nramp2基因与铁转运有关。Nramp2产生两种选择性剪接的mRNA,它们在3'非翻译区因存在或不存在铁反应元件(IRE)而有所不同,并编码两种具有不同羧基末端的蛋白质。制备了针对含有Nramp2羧基或氨基末端的Nramp2融合蛋白的抗血清,这些抗血清有助于区分两种Nramp2蛋白异构体(IRE:异构体I;非IRE:异构体II)。这些抗体用于确定Nramp2在正常组织中的细胞和亚细胞定位,并研究饮食缺铁可能产生的调节作用。对完整器官膜组分进行的免疫印迹实验表明,Nramp2在整个小肠中低水平表达,在肾脏中表达水平较高。饮食缺铁仅导致十二指肠近端部分的Nramp2异构体I显著上调,而小肠其余部分和肾脏中的表达在饮食缺铁时基本保持不变。在十二指肠近端,组织切片的免疫染色研究表明,Nramp2蛋白在缺铁条件下大量表达,仅限于绒毛,隐窝中不存在。在绒毛中,染色仅限于黏膜的柱状吸收上皮(肠上皮细胞),在分泌黏液的杯状细胞或固有层中无表达。Nramp2在绒毛顶端三分之二处表达最强,在肠上皮细胞顶端极的刷状缘处非常强烈,而这些细胞的基底外侧膜对Nramp2呈阴性。这些结果强烈表明,Nramp2确实负责十二指肠中不依赖转铁蛋白的铁摄取。本文在机体铁获取的整体机制背景下讨论了这些发现。

相似文献

[1]
Cellular and subcellular localization of the Nramp2 iron transporter in the intestinal brush border and regulation by dietary iron.

Blood. 1999-6-15

[2]
The Nramp2/DMT1 iron transporter is induced in the duodenum of microcytic anemia mk mice but is not properly targeted to the intestinal brush border.

Blood. 2000-12-1

[3]
Nramp 2 (DCT1/DMT1) expressed at the plasma membrane transports iron and other divalent cations into a calcein-accessible cytoplasmic pool.

J Biol Chem. 2000-11-17

[4]
Localization of iron transport and regulatory proteins in human cells.

QJM. 2000-9

[5]
Expression of the iron transporter DMT1 in kidney from normal and anemic mk mice.

Kidney Int. 2002-7

[6]
Heterologous expression, functional characterization and localization of two isoforms of the monkey iron transporter Nramp2.

Biochem J. 2000-7-1

[7]
The effect of intracellular iron concentration and nitrogen monoxide on Nramp2 expression and non-transferrin-bound iron uptake.

Eur J Biochem. 1999-7

[8]
Expression of the two mRNA isoforms of the iron transporter Nramp2/DMTI in mice and function of the iron responsive element.

Biochem J. 2002-5-1

[9]
The human Nramp2 gene: characterization of the gene structure, alternative splicing, promoter region and polymorphisms.

Blood Cells Mol Dis. 1998-6

[10]
The iron transport protein NRAMP2 is an integral membrane glycoprotein that colocalizes with transferrin in recycling endosomes.

J Exp Med. 1999-3-1

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