Issue 5, 2016
From the journal:

Organic & Biomolecular Chemistry

Comparison of strategies for non-perturbing labeling of α-synuclein to study amyloidogenesis

Conor M. Haney,a   Rebecca F. Wissner,a   John B. Warner,a   Yanxin J. Wang,a   John J. Ferrie,a   Dustin J. Covell,b   Richard J. Karpowicz, Jr.,b   Virginia M.-Y. Leeb  and  E. James Petersson*a  

* Corresponding authors

a Department of Chemistry, University of Pennsylvania, 213 South 34th Street, Philadelphia, PA 19104, USA
E-mail: ejpetersson@sas.upenn.edu
Tel: +1-215-746-2221

b Center for Neurodegenerative Disease Research, University of Pennsylvania, 3600 Spruce Street, Philadelphia, PA 19104, USA

Abstract

Characterization of the amyloidogenic Parkinson's disease protein α-synuclein (αS) has proven difficult due to its structural plasticity. Here, we present a number of complementary methods to site-specifically introduce fluorescent probes to examine αS fibril formation and cellular uptake. By using various combinations of conventional Cys modification, amber codon suppression, transferase mediated N-terminal modification, and native chemical ligation, several variants of singly- and doubly-labeled αS were produced. We validated the nonperturbative nature of the label by a combination of in vitro aggregation kinetics measurements and imaging of the resulting fibrils. The labeled αS can then be used to monitor conformational changes during fibril formation or cellular uptake of αS fibrils in models of disease propagation.

Graphical abstract: Comparison of strategies for non-perturbing labeling of α-synuclein to study amyloidogenesis

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Article information

DOI
https://doi.org/10.1039/C5OB02329G
Article type
Paper
Submitted
12 Nov 2015
Accepted
14 Dec 2015
First published
22 Dec 2015

Org. Biomol. Chem., 2016,14, 1584-1592

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Comparison of strategies for non-perturbing labeling of α-synuclein to study amyloidogenesis

C. M. Haney, R. F. Wissner, J. B. Warner, Y. J. Wang, J. J. Ferrie, D. J. Covell, R. J. Karpowicz, V. M.-Y. Lee and E. James Petersson, Org. Biomol. Chem., 2016, 14, 1584 DOI: 10.1039/C5OB02329G

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