Conformational properties of the SDS-bound state of alpha-synuclein probed by limited proteolysis: unexpected rigidity of the acidic C-terminal tail

Patrizia Polverino de Laureto; Laura Tosatto; Erica Frare; Oriano Marin; Vladimir N Uversky; Angelo Fontana

doi:10.1021/bi052614s

Conformational properties of the SDS-bound state of alpha-synuclein probed by limited proteolysis: unexpected rigidity of the acidic C-terminal tail

Biochemistry. 2006 Sep 26;45(38):11523-31. doi: 10.1021/bi052614s.

Authors

Patrizia Polverino de Laureto¹, Laura Tosatto, Erica Frare, Oriano Marin, Vladimir N Uversky, Angelo Fontana

Affiliation

¹ CRIBI Biotechnology Centre, University of Padua, Viale G. Colombo 3, 35121 Padua, Italy.

PMID: 16981712
DOI: 10.1021/bi052614s

Abstract

Alpha-synuclein (alpha-syn) is a "natively unfolded" protein constituting the major component of intracellular inclusions in several neurodegenerative disorders. Here, we describe proteolysis experiments conducted on human alpha-syn in the presence of SDS micelles. Our aim was to unravel molecular features of micelle-bound alpha-syn using the limited proteolysis approach. The nonspecific proteases thermolysin and proteinase K, as well as the Glu-specific V8-protease, were used as proteolytic probes. While alpha-syn at neutral pH is easily degraded to a variety of relatively small fragments, in the presence of 10 mM SDS the proteolysis of the protein is rather selective. Complementary fragments 1-111 and 112-140, 1-113 and 114-140, and 1-123 and 124-140 are obtained when thermolysin, proteinase K, and V8 protease, respectively, are used. These results are in line with a conformational model of alpha-syn in which it acquires a folded helical structure in the N-terminal region in its membrane-bound state. At the same time, they indicate that the C-terminal portion of the molecule is rather rigid, as seen in its relative resistance to extensive proteolytic degradation. It is likely that, under the specific experimental conditions of proteolysis in the presence of SDS, the negatively charged C-terminal region can be rigidified by binding a calcium ion, as shown before with intact alpha-syn. In this study, some evidence of calcium binding properties of isolated C-terminal fragments 112-140, 114-140, and 124-140 was obtained by mass spectrometry measurements, since molecular masses for calcium-loaded fragments were obtained. Our results indicate that the C-terminal portion of the membrane-bound alpha-syn is quite rigid and structured, at variance from current models of the membrane-bound protein deduced mostly from NMR. Considering that the aggregation process of alpha-syn is modulated by its C-terminal tail, the results of this study may provide useful insights into the behavior of alpha-syn in a membrane-mimetic environment.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Amino Acid Sequence
Circular Dichroism
Endopeptidase K / metabolism
Humans
Models, Biological
Molecular Sequence Data
Peptide Fragments / chemistry
Peptide Fragments / metabolism
Protein Binding
Protein Processing, Post-Translational*
Protein Structure, Secondary
Sodium Dodecyl Sulfate / metabolism*
Spectrometry, Mass, Electrospray Ionization
Structure-Activity Relationship
Thermolysin / metabolism
alpha-Synuclein / chemistry*
alpha-Synuclein / metabolism*

Substances

Peptide Fragments
alpha-Synuclein
Sodium Dodecyl Sulfate
Endopeptidase K
Thermolysin