Induced Dimerization of the Amyloid Precursor Protein Leads to Decreased Amyloid-β Protein Production

Eggert, Simone; Midthune, Brea; Cottrell, Barbara A.; Koo, Edward H.

doi:10.1074/jbc.m109.038646

Cited by 87 publications

(155 citation statements)

References 54 publications

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“…APP and its mammalian homologs, the APP-like proteins, can form intracellular homo-and heterodimers; although APP is monomeric in solution in vitro, it dimerizes in the presence of heparin (Gralle et al, 2006), thus possibly reducing Ab generation (Eggert et al, 2009). The E2 domain of APP-like protein 1 crystallizes as a dimer, and a heparin hexasaccharide soaked into the crystal is bound asymmetrically within the dimer, making different contacts with the two protein monomers; one heparin oligosaccharide is bound to each dimer (3QMK) (Xue et al, 2011).…”

Section: F Protein Aggregation In the Nervous Systemmentioning

confidence: 99%

Pharmacology of Heparin and Related Drugs

et al. 2015

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Section: F Protein Aggregation In the Nervous Systemmentioning

confidence: 99%

Pharmacology of Heparin and Related Drugs

et al. 2015

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“…Surprisingly, A␤ could not be detected for the K28E mutant in cultured cells and the cell-free assay system by SDS-PAGE (data not shown). This may reflect a potential alteration of the folding of Lys-28 mutant A␤ peptides (45), which could possibly have affected their detectability in some of the previous reports (22,46,47 FIGURE 4. Validation of cell-free assay system concerning the cleavage specificity of purified ␥-secretase on mutant APP C-terminal fragment based C100-His 6 substrates.…”

Section: Fad Mutants In the ␥-Secretase Cleavage Site Regionmentioning

confidence: 99%

“…This region is known to be critical for A␤ aggregation (19 -21), and aggregation inhibitors interacting with this region also act as GSMs (18). However, a recent study demonstrated that dimerization per se might not be a factor that determines ␥-secretase cleavage specificity (22), and whether GXXXG mutants inhibit dimerization is controversial (23). In addition, the lack of a consistent response to GSMs regarding an inversely correlated production of A␤ 42 and A␤ 38 by PS FAD mutants observed earlier argued against a strict precursor-product relationship between A␤ 42 and A␤ 38 (24,25).…”

mentioning

confidence: 99%

β-Amyloid Precursor Protein Mutants Respond to γ-Secretase Modulators

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Gutsmiedl

Fukumori

et al. 2010

Journal of Biological Chemistry

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Pathogenic generation of the 42-amino acid variant of the amyloid ␤-peptide (A␤) by ␤-and ␥-secretase cleavage of the ␤-amyloid precursor protein (APP) is believed to be causative for Alzheimer disease (AD). Lowering of A␤ 42 production by ␥-secretase modulators (GSMs) is a hopeful approach toward AD treatment. The mechanism of GSM action is not fully understood. Moreover, whether GSMs target the A␤ domain is controversial. To further our understanding of the mode of action of GSMs and the cleavage mechanism of ␥-secretase, we analyzed mutations located at different positions of the APP transmembrane domain around or within the A␤ domain regarding their response to GSMs. We found that A␤ 42 -increasing familial AD mutations of the ␥-secretase cleavage site domain responded robustly to A␤ 42 -lowering GSMs, especially to the potent compound GSM-1, irrespective of the amount of A␤ 42 produced. We thus expect that familial AD patients carrying mutations at the ␥-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 A␤ species (A␤ 41 , A␤ 39 ) could also be lowered besides A␤ 42 . Moreover, certain mutations simultaneously increased A␤ 42 and the shorter peptide A␤ 38 , arguing that the proposed precursor-product relationship of these A␤ species is not general. Finally, mutations of residues in the proposed GSM-binding site implicated in A␤ 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.Alzheimer disease (AD) 3 is the most common neurodegenerative disorder worldwide. The ␤-amyloid precursor protein (APP), a type I membrane protein, plays a central role in the pathogenesis of the disease (1). Sequential cleavage of APP by ␤-and ␥-secretase generates the amyloid-␤ (A␤) peptide, which deposits as plaques in the brain of affected patients and represents one of the principal pathological hallmarks of the disease (1). ␥-Secretase is an intramembrane-cleaving protease complex, which cleaves the APP transmembrane domain (TMD) in a progressive, stepwise manner via cleavages at the ⑀-, -, and ␥-sites until it is sufficiently shortened to allow the release of A␤ from the membrane (2-4). A␤ peptides generated by ␥-secretase cleavage differ in their C termini. The major product released is A␤ 40 , whereas A␤ 38 and A␤ 42 represent minor species (1). The highly aggregation-prone, neurotoxic A␤ 42 is believed to be causative for AD by initiating a cascade of pathogenic events, which ultimately causes neurodegeneration and dementia (1). Increased production of A␤ 42 underlies the vast majority of mutations associated with familial AD (FAD), which manifests with a very early disease onset. The majority of FAD mutations have been found in PS1, the catalytic subunit of ␥-secretase (5), whereas only a few mutations were found in its h...

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“…1) (Spencer et al, 1993;Eggert et al, 2009). In contrast to cross-linking antibodies, AP20187 is permeable and is able to target intracellular Fv-PrP.…”

Section: Enforced Prpmentioning

confidence: 99%

PrP^CHomodimerization Stimulates the Production of PrP^CCleaved Fragments PrPN1 and PrPC1

et al. 2012

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An endoproteolytic cleavage termed ␣-cleavage between residues 111/112 is a characteristic feature of the cellular prion protein (PrP C ). This cleavage generates a soluble N-terminal fragment (PrPN1) and a glycosylphosphatidylinositol-anchored C-terminal fragment (PrPC1). Independent studies demonstrate that modulating PrP C ␣-cleavage represents a potential therapeutic strategy in prion diseases. The regulation of PrP C ␣-cleavage is unclear. The only known domain that is essential for the ␣-cleavage to occur is a hydrophobic domain (HD). Importantly, the HD is also essential for the formation of PrP C homodimers. To explore the role of PrP C homodimerization on the ␣-cleavage, we used a well described inducible dimerization strategy whereby a chimeric PrP C composed of a modified FK506-binding protein (Fv) fused with PrP C and termed Fv-PrP is incubated in the presence of a dimerizer AP20187 ligand. We show that homodimerization leads to a considerable increase of PrP C ␣-cleavage in cultured cells and release of PrPN1 and PrPC1. Interestingly, enforced homodimerization increased PrP C levels at the plasma membrane, and preventing PrP C trafficking to the cell surface inhibited dimerization-induced ␣-cleavage. These observations were confirmed in primary hippocampal neurons from transgenic mice expressing Fv-PrP. The proteases responsible for the ␣-cleavage are still elusive, and in contrast to initial studies we confirm more recent investigations that neither ADAM10 nor ADAM17 are involved. Importantly, PrPN1 produced after PrP C homodimerization protects against toxic amyloid-␤ (A␤) oligomers. Thus, our results show that PrP C homodimerization is an important regulator of PrP C ␣-cleavage and may represent a potential therapeutic avenue against A␤ toxicity in Alzheimer's disease.

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Induced Dimerization of the Amyloid Precursor Protein Leads to Decreased Amyloid-β Protein Production

Cited by 87 publications

References 54 publications

Pharmacology of Heparin and Related Drugs

Pharmacology of Heparin and Related Drugs

β-Amyloid Precursor Protein Mutants Respond to γ-Secretase Modulators

PrP^CHomodimerization Stimulates the Production of PrP^CCleaved Fragments PrPN1 and PrPC1

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Induced Dimerization of the Amyloid Precursor Protein Leads to Decreased Amyloid-β Protein Production

Cited by 87 publications

References 54 publications

Pharmacology of Heparin and Related Drugs

Pharmacology of Heparin and Related Drugs

β-Amyloid Precursor Protein Mutants Respond to γ-Secretase Modulators

PrPCHomodimerization Stimulates the Production of PrPCCleaved Fragments PrPN1 and PrPC1

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PrP^CHomodimerization Stimulates the Production of PrP^CCleaved Fragments PrPN1 and PrPC1