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铁调节蛋白-1 对阿尔茨海默病淀粉样前体蛋白转录本的选择性翻译调控。

Selective translational control of the Alzheimer amyloid precursor protein transcript by iron regulatory protein-1.

机构信息

Neurochemistry Laboratory, Department of Psychiatry-Neuroscience, Massachusetts General Hospital, Harvard Medical School, Charlestown, Massachusetts 02129, USA.

出版信息

J Biol Chem. 2010 Oct 8;285(41):31217-32. doi: 10.1074/jbc.M110.149161. Epub 2010 Jun 17.

DOI:10.1074/jbc.M110.149161
PMID:20558735
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2951196/
Abstract

Iron influx increases the translation of the Alzheimer amyloid precursor protein (APP) via an iron-responsive element (IRE) RNA stem loop in its 5'-untranslated region. Equal modulated interaction of the iron regulatory proteins (IRP1 and IRP2) with canonical IREs controls iron-dependent translation of the ferritin subunits. However, our immunoprecipitation RT-PCR and RNA binding experiments demonstrated that IRP1, but not IRP2, selectively bound the APP IRE in human neural cells. This selective IRP1 interaction pattern was evident in human brain and blood tissue from normal and Alzheimer disease patients. We computer-predicted an optimal novel RNA stem loop structure for the human, rhesus monkey, and mouse APP IREs with reference to the canonical ferritin IREs but also the IREs encoded by erythroid heme biosynthetic aminolevulinate synthase and Hif-2α mRNAs, which preferentially bind IRP1. Selective 2'-hydroxyl acylation analyzed by primer extension analysis was consistent with a 13-base single-stranded terminal loop and a conserved GC-rich stem. Biotinylated RNA probes deleted of the conserved CAGA motif in the terminal loop did not bind to IRP1 relative to wild type probes and could no longer base pair to form a predicted AGA triloop. An AGU pseudo-triloop is key for IRP1 binding to the canonical ferritin IREs. RNA probes encoding the APP IRE stem loop exhibited the same high affinity binding to rhIRP1 as occurs for the H-ferritin IRE (35 pm). Intracellular iron chelation increased binding of IRP1 to the APP IRE, decreasing intracellular APP expression in SH-SY5Y cells. Functionally, shRNA knockdown of IRP1 caused increased expression of neural APP consistent with IRP1-APP IRE-driven translation.

摘要

铁的流入通过其 5'非翻译区中的一个铁反应元件 (IRE) RNA 茎环增加阿尔茨海默病淀粉样前体蛋白 (APP) 的翻译。铁调节蛋白 (IRP1 和 IRP2) 与典型 IRE 之间的同等调节相互作用控制铁蛋白亚基的铁依赖性翻译。然而,我们的免疫沉淀 RT-PCR 和 RNA 结合实验表明,IRP1 但不是 IRP2,选择性地与人神经细胞中的 APP IRE 结合。这种选择性的 IRP1 相互作用模式在来自正常和阿尔茨海默病患者的人脑和血液组织中是明显的。我们计算机预测了人类、恒河猴和小鼠 APP IRE 的最佳新型 RNA 茎环结构,参考了典型的铁蛋白 IRE,以及优先与 IRP1 结合的红细胞血红素生物合成氨基酮戊酸合酶和 Hif-2α mRNA 编码的 IRE。通过引物延伸分析进行的选择性 2'-羟基酰化分析与 13 个碱基的单链末端环和保守的 GC 丰富的茎一致。与野生型探针相比,缺失末端环中保守的 CAGA 基序的生物素化 RNA 探针不能与 IRP1 结合,并且不能再形成预测的 AGA 三链环。AGU 假三链环是 IRP1 与典型铁蛋白 IRE 结合的关键。编码 APP IRE 茎环的 RNA 探针与 H 铁蛋白 IRE(35 pm)一样对 rhIRP1 表现出相同的高亲和力结合。细胞内铁螯合增加了 IRP1 与 APP IRE 的结合,减少了 SH-SY5Y 细胞中的细胞内 APP 表达。在功能上,IRP1 的 shRNA 敲低导致神经 APP 的表达增加,与 IRP1-APP IRE 驱动的翻译一致。

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