Abstract

Pathogenic generation of the 42-amino acid variant of the amyloid beta-peptide (Abeta) by beta- and gamma-secretase cleavage of the beta-amyloid precursor protein (APP) is believed to be causative for Alzheimer disease (AD). Lowering of Abeta(42) production by gamma-secretase modulators (GSMs) is a hopeful approach toward AD treatment. The mechanism of GSM action is not fully understood. Moreover, whether GSMs target the Abeta domain is controversial. To further our understanding of the mode of action of GSMs and the cleavage mechanism of gamma-secretase, we analyzed mutations located at different positions of the APP transmembrane domain around or within the Abeta domain regarding their response to GSMs. We found that Abeta(42)-increasing familial AD mutations of the gamma-secretase cleavage site domain responded robustly to Abeta(42)-lowering GSMs, especially to the potent compound GSM-1, irrespective of the amount of Abeta(42) produced. We thus expect that familial AD patients carrying mutations at the gamma-secretase cleavage sites of APP should respond to GSM-based therapeutic approaches. Systematic phenylalanine-scanning mutagenesis of this region revealed a high permissiveness to GSM-1 and demonstrated a complex mechanism of GSM action as other Abeta species (Abeta(41), Abeta(39)) could also be lowered besides Abeta(42). Moreover, certain mutations simultaneously increased Abeta(42) and the shorter peptide Abeta(38), arguing that the proposed precursor-product relationship of these Abeta species is not general. Finally, mutations of residues in the proposed GSM-binding site implicated in Abeta(42) generation (Gly-29, Gly-33) and potentially in GSM-binding (Lys-28) were also responsive to GSMs, a finding that may question APP substrate targeting of GSMs.

Highlights

  • The relative change in the A␤42/A␤total and A␤38/A␤total ratio as determined by A␤ immunoassay for each mutant as compared with WT is indicated by arrows

  • The magnitude of response to GSMs as compared with WT is indicated (WT response is equivalent to ϩϩϩ)

  • All responses summarized in this table refer to GSM-1, except for some mutants in the proposed GSM-binding site

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Summary

Introduction

The Gly mutants were responsive to GSM-1, which effectively lowered A␤42 for G29A and G33A, while increasing A␤38 levels. TMD interactions, whether involving dimerization or not Because the GXXXG mutant substrates give rise to mutated A␤ peptides, whose altered biochemical properties may affect the levels detectable in cultured cells downstream of production, we analyzed these using our recently described validated cell-free in vitro system consisting of purified ␥-secretase and purified APP substrate (28).

Results
Conclusion

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