Visualizing alpha‐synuclein and iron deposition in M83 mouse model of Parkinson's disease in vivo

Author:

Straumann Nadja1,Combes Benjamin F.1,Dean Ben Xose Luis2,Sternke‐Hoffmann Rebecca3,Gerez Juan A.4,Dias Ines5,Chen Zhenyue2,Watts Benjamin6,Rostami Iman7,Shi Kuangyu8,Rominger Axel8,Baumann Christian R.5,Luo Jinghui3,Noain Daniela5,Nitsch Roger M.1,Okamura Nobuyuki9,Razansky Daniel2,Ni Ruiqing128ORCID

Affiliation:

1. Institute for Regenerative Medicine University of Zurich Zurich Switzerland

2. Institute for Biomedical Engineering University of Zurich & ETH Zurich Zurich Switzerland

3. Department of Biology and Chemistry Paul Scherrer Institute Villigen Switzerland

4. Laboratory of Physical Chemistry, Department of Chemistry and Applied Biosciences ETH Zurich Zurich Switzerland

5. Neurology Department University Hospital Zurich Zurich Switzerland

6. Photon Science Division Paul Scherrer Institute Villigen Switzerland

7. Microscopic Anatomy and Structural Biology University of Bern Bern Switzerland

8. Department of Nuclear Medicine, Inselspital Bern University Hospital, University of Bern Bern Switzerland

9. Division of Pharmacology, Faculty of Medicine Tohoku Medical and Pharmaceutical University Sendai Japan

Abstract

AbstractAbnormal alpha‐synuclein (αSyn) and iron accumulation in the brain play an important role in Parkinson's disease (PD). Herein, we aim to visualize αSyn inclusions and iron deposition in the brains of M83 (A53T) mouse models of PD in vivo. The fluorescent pyrimidoindole derivative THK‐565 probe was characterized by means of recombinant fibrils and brains from 10‐ to 11‐month‐old M83 mice. Concurrent wide‐field fluorescence and volumetric multispectral optoacoustic tomography (vMSOT) imaging were subsequently performed in vivo. Structural and susceptibility weighted imaging (SWI) magnetic resonance imaging (MRI) at 9.4 T as well as scanning transmission x‐ray microscopy (STXM) were performed to characterize the iron deposits in the perfused brains. Immunofluorescence and Prussian blue staining were further performed on brain slices to validate the detection of αSyn inclusions and iron deposition. THK‐565 showed increased fluorescence upon binding to recombinant αSyn fibrils and αSyn inclusions in post‐mortem brain slices from patients with PD and M83 mice. Administration of THK‐565 in M83 mice showed higher cerebral retention at 20 and 40 min post‐intravenous injection by wide‐field fluorescence compared to nontransgenic littermate mice, in congruence with the vMSOT findings. SWI/phase images and Prussian blue indicated the accumulation of iron deposits in the brains of M83 mice, presumably in the Fe3+ form, as evinced by the STXM results. In conclusion, we demonstrated in vivo mapping of αSyn by means of noninvasive epifluorescence and vMSOT imaging and validated the results by targeting the THK‐565 label and SWI/STXM identification of iron deposits in M83 mouse brains ex vivo.

Funder

National Institutes of Health

Innosuisse - Schweizerische Agentur für Innovationsförderung

Novartis Stiftung für Medizinisch-Biologische Forschung

Schweizerischer Nationalfonds zur Förderung der Wissenschaftlichen Forschung

Olga Mayenfisch Stiftung

Parkinson Schweiz

Fondation Gustave et Simone Prévot

Publisher

Wiley

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