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α-Synuclein propagates from mouse brain to grafted dopaminergic neurons and seeds aggregation in cultured human cells
Christian Hansen, … , Jia-Yi Li, Patrik Brundin
Christian Hansen, … , Jia-Yi Li, Patrik Brundin
Published January 18, 2011
Citation Information: J Clin Invest. 2011;121(2):715-725. https://doi.org/10.1172/JCI43366.
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Research Article Neuroscience

α-Synuclein propagates from mouse brain to grafted dopaminergic neurons and seeds aggregation in cultured human cells

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Abstract

Post-mortem analyses of brains from patients with Parkinson disease who received fetal mesencephalic transplants show that α-synuclein–containing (α-syn–containing) Lewy bodies gradually appear in grafted neurons. Here, we explored whether intercellular transfer of α-syn from host to graft, followed by seeding of α-syn aggregation in recipient neurons, can contribute to this phenomenon. We assessed α-syn cell-to-cell transfer using microscopy, flow cytometry, and high-content screening in several coculture model systems. Coculturing cells engineered to express either GFP– or DsRed-tagged α-syn resulted in a gradual increase in double-labeled cells. Importantly, α-syn–GFP derived from 1 neuroblastoma cell line localized to red fluorescent aggregates in other cells expressing DsRed–α-syn, suggesting a seeding effect of transmitted α-syn. Extracellular α-syn was taken up by cells through endocytosis and interacted with intracellular α-syn. Next, following intracortical injection of recombinant α-syn in rats, we found neuronal uptake was attenuated by coinjection of an endocytosis inhibitor. Finally, we demonstrated in vivo transfer of α-syn between host cells and grafted dopaminergic neurons in mice overexpressing human α-syn. In summary, intercellularly transferred α-syn interacts with cytoplasmic α-syn and can propagate α-syn pathology. These results suggest that α-syn propagation is a key element in the progression of Parkinson disease pathology.

Authors

Christian Hansen, Elodie Angot, Ann-Louise Bergström, Jennifer A. Steiner, Laura Pieri, Gesine Paul, Tiago F. Outeiro, Ronald Melki, Pekka Kallunki, Karina Fog, Jia-Yi Li, Patrik Brundin

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Figure 2

Intercellular propagation of α-syn in HEK cell culture.

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Intercellular propagation of α-syn in HEK cell culture.
(A) Epifluoresce...
(A) Epifluorescence microscopy: representative picture showing double-labeled HEK cells after 5 days of coculture of stable HEK cell lines expressing α-syn fused to either GFP or DsRed. Original magnification, ×40. (B) Confocal microscopy: representative picture showing double-labeled HEK cells after 5 days of coculture of stable HEK cell lines expressing α-syn fused to either GFP or DsRed. Scale bars: 5 μM. Arrows represent double-labeled cells. Arrowheads represent aggregates of transferred α-syn. (C) Representative illustrations of α-syn transfer between cells as evaluated by FACS analysis. Cells expressing α-syn–DsRed or GFP–α-syn were analyzed separately (upper panels) and mixed together just prior to the analysis (negative control, lower left panel) or after 7 days of coculture (lower right panel). (D) Quantification from 20,000 cells in FACS analysis after 0, 1, 2, 4, or 7 days of coculture of α-syn–DsRed– and GFP–α-syn–expressing HEK cells (n = 3). Error bars represent SD.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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