α-Synuclein–Confocal Nanoscanning (ASYN-CONA), a Bead-Based Assay for Detecting Early-Stage α-Synuclein Aggregation | Zendy

Irene PérezPi | Zendy; David Evans | Zendy; Mathew H. Horrocks | Zendy; Nhan T. Pham | Zendy; Karamjit Singh Dolt | Zendy; Joanna Koszela | Zendy; Tilo Kunath | Zendy; Manfred Auer | Zendy

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α-Synuclein–Confocal Nanoscanning (ASYN-CONA), a Bead-Based Assay for Detecting Early-Stage α-Synuclein Aggregation

Author(s) -

Irene PérezPi,

David Evans,

Mathew H. Horrocks,

Nhan T. Pham,

Karamjit Singh Dolt,

Joanna Koszela,

Tilo Kunath,

Manfred Auer

Publication year - 2019

Publication title -

analytical chemistry

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 2.117

H-Index - 332

eISSN - 1520-6882

pISSN - 0003-2700

DOI - 10.1021/acs.analchem.8b03842

Subject(s) - chemistry , fluorescence , confocal microscopy , confocal , biophysics , monomer , fibril , synucleinopathies , protein aggregation , thioflavin , total internal reflection fluorescence microscope , bead , fluorescence lifetime imaging microscopy , alpha synuclein , amyloid (mycology) , biochemistry , polymer , microbiology and biotechnology , parkinson's disease , organic chemistry , materials science , mathematics , membrane , pathology , composite material , biology , geometry , quantum mechanics , medicine , physics , disease , alzheimer's disease , inorganic chemistry

α-Synuclein fibrils are considered a hallmark of Parkinson's disease and other synucleinopathies. However, small oligomers that formed during the early stages of α-synuclein aggregation are thought to be the main toxic species causing disease. The formation of α-synuclein oligomers has proven difficult to follow, because of the heterogeneity and transient nature of the species formed. Here, a novel bead-based aggregation assay for monitoring the earliest stages of α-synuclein oligomerization, α-Synuclein-Confocal Nanoscanning (ASYN-CONA), is presented. The α-synuclein A91C single cysteine mutant is modified with a trifunctional chemical tag, which allows simultaneous fluorescent labeling with a green dye (tetramethylrhodamine, TMR) and attachment to microbeads. Beads with bound TMR-labeled α-synuclein are then incubated with a red dye (Cy5)-labeled variant of α-synuclein A91C, and EtOH (20%) to induce aggregation. Aggregation is detected by confocal scanning imaging, below the equatorial plane of the beads, which is known as the CONA technique. On-bead TMR-labeled α-synuclein and aggregated Cy5-labeled α-synuclein from the solution are quantitatively monitored in parallel by detection of fluorescent halos or "rings". α-Synuclein on-bead oligomerization results in a linear increase of red bead ring fluorescence intensity over a period of 5 h. Total internal reflection fluorescence microscopy was performed on oligomers cleaved from the beads, and it revealed that (i) oligomers are sufficiently stable in solution to investigate their composition, consisting of 6 ± 1 monomer units, and (ii) oligomers containing a mean of 15 monomers bind Thioflavin-T. Various known inhibitors of α-synuclein aggregation were used to validate the ASYN-CONA assay for drug screening. Baicalein, curcumin, and rifampicin showed concentration-dependent inhibition of the α-synuclein aggregation and the IC 50 (the concentration of the compound at which the maxiumum intensity was reduced by one-half) were calculated.

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