4.5 Article

Quantification of α-synuclein binding to lipid vesicles using fluorescence correlation spectroscopy

Journal

BIOPHYSICAL JOURNAL
Volume 90, Issue 12, Pages 4692-4700

Publisher

CELL PRESS
DOI: 10.1529/biophysj.105.079251

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Funding

  1. NIA NIH HHS [R21 AG026650, R01 AG019391, R01 AG025440-01A1, R01 AG025440, 1 R21 AG26650, R01 AG019391-06, R37 AG019391, AG19391] Funding Source: Medline
  2. NIBIB NIH HHS [9 P41 EB001976, P41 EB001976] Funding Source: Medline

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alpha-Synuclein (alpha S) is a soluble synaptic protein that is the major proteinaceous component of insoluble fibrillar Lewy body deposits that are the hallmark of Parkinson's disease. The interaction of aS with synaptic vesicles is thought to be critical both to its normal function as well as to its pathological role in Parkinson's disease. We demonstrate the use of fluorescence correlation spectroscopy as a tool for rapid and quantitative analysis of the binding of alpha S to large unilamellar vesicles of various lipid compositions. We find that aS binds preferentially to vesicles containing acidic lipids, and that this interaction can be blocked by increasing the concentration of NaCl in solution. Negative charge is not the only factor determining binding, as we clearly observe binding to vesicles composed entirely of zwitterionic lipids. Additionally, we find enhanced binding to lipids with less bulky headgroups. Quanti. cation of the protein-to-lipid ratio required for binding to different lipid compositions, combined with other data in the literature, yields an upper bound estimate for the number of lipid molecules required to bind each individual molecule of aS. Our results demonstrate that fluorescence correlation spectroscopy provides a powerful tool for the quantitative characterization of alpha S-lipid interactions.

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