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双标记淀粉样前体蛋白揭示其N端和C端片段的不同运输途径。

Dual-tagged amyloid-β precursor protein reveals distinct transport pathways of its N- and C-terminal fragments.

作者信息

Villegas Christine, Muresan Virgil, Ladescu Muresan Zoia

机构信息

Department of Pharmacology and Physiology, New Jersey Medical School, Rutgers, The State University of New Jersey, Newark, NJ 07101-1709, USA.

出版信息

Hum Mol Genet. 2014 Mar 15;23(6):1631-43. doi: 10.1093/hmg/ddt555. Epub 2013 Nov 7.

Abstract

The amyloid-β precursor protein (APP), a type I transmembrane protein genetically associated with Alzheimer's disease, has a complex biology that includes proteolytic processing into potentially toxic fragments, extensive trafficking and multiple, yet poorly-defined functions. We recently proposed that a significant fraction of APP is proteolytically cleaved in the neuronal soma into N- and C-terminal fragments (NTFs and CTFs), which then target independently of each other to separate destinations in the cell. Here, we prove this concept with live imaging and immunolocalization of two dual, N- and C-termini-tagged APP constructs: CFP-APP-YFP [containing the fluorescent tags, cyan fluorescent protein (CFP) and yellow fluorescent protein (YFP)] and FLAG-APP-Myc. When expressed at low levels in neuronal cells, these constructs are processed into differently tagged NTFs and CTFs that reveal distinct distributions and characteristics of transport. Like the endogenous N- and C-terminal epitopes of APP, the FLAG-tagged NTFs are present in trains of vesicles and tubules that localize to short filaments, which often immunostain for acetylated tubulin, whereas the Myc-tagged CTFs are detected on randomly distributed vesicle-like structures. The experimental treatments that selectively destabilize the acetylated microtubules abrogate the distribution of NTFs along filaments, without altering the random distribution of CTFs. These results indicate that the NTFs and CTFs are recruited to distinct transport pathways and reach separate destinations in neurons, where they likely accomplish functions independent of the parental, full-length APP. They also point to a compartment associated with acetylated microtubules in the neuronal soma--not the neurite terminals--as a major site of APP cleavage, and segregation of NTFs from CTFs.

摘要

淀粉样前体蛋白(APP)是一种与阿尔茨海默病存在遗传关联的I型跨膜蛋白,其生物学特性复杂,包括蛋白水解加工成潜在毒性片段、广泛的运输以及多种定义尚不明确的功能。我们最近提出,相当一部分APP在神经元胞体中被蛋白水解切割成N端和C端片段(NTFs和CTFs),然后它们彼此独立地靶向细胞内不同的目的地。在此,我们通过对两种带有N端和C端双重标签的APP构建体进行实时成像和免疫定位来证明这一概念:CFP-APP-YFP [含有荧光标签,青色荧光蛋白(CFP)和黄色荧光蛋白(YFP)]和FLAG-APP-Myc。当在神经元细胞中低水平表达时,这些构建体会被加工成带有不同标签的NTFs和CTFs,它们显示出不同的运输分布和特征。与APP的内源性N端和C端表位一样,带有FLAG标签的NTFs存在于定位于短细丝的小泡和小管序列中,这些细丝通常对乙酰化微管进行免疫染色,而带有Myc标签的CTFs则在随机分布的类小泡结构上被检测到。选择性破坏乙酰化微管的实验处理消除了NTFs沿细丝的分布,而不改变CTFs的随机分布。这些结果表明,NTFs和CTFs被招募到不同的运输途径并在神经元中到达不同的目的地,在那里它们可能独立于亲本全长APP完成功能。它们还指出,神经元胞体中与乙酰化微管相关的区室——而非神经突末端——是APP切割以及NTFs与CTFs分离的主要部位。

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