Stabilizing capping motif for β-hairpins and sheets

Kier, Brandon L.; Shu, Irene; Eidenschink, Lisa A.; Andersen, Niels H.

doi:10.1073/pnas.0913534107

Cited by 80 publications

(169 citation statements)

References 43 publications

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“…The concentration range examined was 0 – 8 or 0 –20 vol-% HFIP. In most cases, there was an increase in β structure stability observed at 8 or 20 vol-% HFIP as has previously been observed for other β hairpins 63–67 .…”

Section: Methodssupporting

confidence: 79%

Binding interactions of agents that alter α-synuclein aggregation

et al. 2015

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Further examination of peptides with well-folded antiparallel β strands as inhibitors of amyloid formation from α-synuclein has resulted in more potent inhibitors. Several of these had multiple Tyr residues and represent a new lead for inhibitor design by small peptides that do not divert α-synuclein to non-amyloid aggregate formation. The most potent inhibitor obtained in this study is a backbone cyclized version of a previously studied β hairpin, designated as WW2, with a cross-strand Trp/Trp cluster. The cyclization was accomplished by adding a d-Pro-l-Pro turn locus across strand termini. At a 2:1 peptide to α-synuclein ratio, cyclo-WW2 displays complete inhibition of β-structure formation. Trp-bearing antiparallel β-sheets held together by a disulphide bond are also potent inhibitors. 15N HSQC spectra of α-synuclein provided new mechanistic details. The time course of 15N HSQC spectral changes observed during β-oligomer formation has revealed which segments of the structure become part of the rigid core of an oligomer at early stages of amyloidogenesis and that the C-terminus remains fully flexible throughout the process. All of the effective peptide inhibitors display binding-associated titration shifts in 15N HSQC spectra of α-synuclein in the C-terminal Q109-E137 segment. Cyclo-WW2, the most potent inhibitor, also displays titration shifts in the G41-T54 span of α-synuclein, an additional binding site. The earliest aggregation event appears to be centered about H50 which is also a binding site for our most potent inhibitor.

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Section: Methodssupporting

confidence: 79%

Binding interactions of agents that alter α-synuclein aggregation

et al. 2015

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“…The location of the relatively close C terminus was not altered due to a stabilizing salt bridge between K25 and D132. In both models, W92 and W103 exhibit an edge-to-face orientation, indicating their importance to stabilize aryl/aryl cross-strand interactions ( 46 ). This is in good agreement with the unsuccessful expression of W92A and W103A, possibly due to a failure of the mutants to acquire the correct folding state.…”

Section: Measurement Of Hemolysissupporting

confidence: 70%

Binding of a pleurotolysin ortholog from Pleurotus eryngii to sphingomyelin and cholesterol-rich membrane domains

Bhat

Kishimoto

Abe

et al. 2013

Journal of Lipid Research

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“…Model b-hairpin peptides with aromatic (and especially Trp) residues have been observed to yield similar CD spectra arising from exciton coupling contribution of Trp side chain. [21,23,40] There were no significant changes in the CD spectra of IV8 and IV8FA in the presence of cofactor, indicating peptides do not undergo any major conformational rearrangement in complex with heme (Supporting Information, Figure S6). Further, binding of heme with the designed peptides produces an induced CD band for heme at the Soret region of the absorption spectra, indicating that the heme is experiencing a chiral environment (Supporting Information, Figure S7).…”

Section: Mukesh Mahajan and Surajit Bhattacharjya*mentioning

confidence: 91%