Amyloid precursor protein–mediated endocytic pathway disruption induces axonal dysfunction and neurodegeneration
Wei Xu, … , William C. Mobley, Chengbiao Wu
Wei Xu, … , William C. Mobley, Chengbiao Wu
Published April 11, 2016
Citation Information: J Clin Invest. 2016;126(5):1815-1833. https://doi.org/10.1172/JCI82409.
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Research Article Neuroscience

Amyloid precursor protein–mediated endocytic pathway disruption induces axonal dysfunction and neurodegeneration

Abstract

The endosome/lysosome pathway is disrupted early in the course of both Alzheimer’s disease (AD) and Down syndrome (DS); however, it is not clear how dysfunction in this pathway influences the development of these diseases. Herein, we explored the cellular and molecular mechanisms by which endosomal dysfunction contributes to the pathogenesis of AD and DS. We determined that full-length amyloid precursor protein (APP) and its β-C-terminal fragment (β-CTF) act though increased activation of Rab5 to cause enlargement of early endosomes and to disrupt retrograde axonal trafficking of nerve growth factor (NGF) signals. The functional impacts of APP and its various products were investigated in PC12 cells, cultured rat basal forebrain cholinergic neurons (BFCNs), and BFCNs from a mouse model of DS. We found that the full-length wild-type APP (APPWT) and β-CTF both induced endosomal enlargement and disrupted NGF signaling and axonal trafficking. β-CTF alone induced atrophy of BFCNs that was rescued by the dominant-negative Rab5 mutant, Rab5S34N. Moreover, expression of a dominant-negative Rab5 construct markedly reduced APP-induced axonal blockage in Drosophila. Therefore, increased APP and/or β-CTF impact the endocytic pathway to disrupt NGF trafficking and signaling, resulting in trophic deficits in BFCNs. Our data strongly support the emerging concept that dysregulation of Rab5 activity contributes importantly to early pathogenesis of AD and DS.

Authors

Wei Xu, April M. Weissmiller, Joseph A. White II, Fang Fang, Xinyi Wang, Yiwen Wu, Matthew L. Pearn, Xiaobei Zhao, Mariko Sawa, Shengdi Chen, Shermali Gunawardena, Jianqing Ding, William C. Mobley, Chengbiao Wu

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Figure 6

APP, APP mutants, or C99 inhibited NGF-induced neurite outgrowth that was rescued by Rab5S34N.

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APP, APP mutants, or C99 inhibited NGF-induced neurite outgrowth that wa...
PC12M cells were transfected with the indicated plasmids and treated with 50 ng/ml NGF for 48 hours. The length and the number of neurites of each cell were measured and quantitated using ImageJ. Representative images are shown in A. The number of the neurites/cell (B) and the average length (C) in each condition are measured, and the results are shown. (DF) Rab5S34N-GFP or Rab5S34N-mCherry was cotransfected with APP-mCherry or Rabex-5–GFP into PC12M cells (D). Cells were then induced for differentiation. The number of the neurites/cell (E) and the average length (F) of each condition were measured, and the results are shown. All P values were calculated using Student’s t test; ***P < 0.001. Scale bars: 20 μm.