Abstract

The central hypothesis underlying our research is that Alzheimer's disease is a multi-gene syndrome in which numerous distinct gene defects (and perhaps certain environmental factors) result in a chronic imbalance between Abeta production and Abeta clearance that leads to the microglial, astrocytic, neuronal and synaptic pathology which produce the symptoms of dementia. Based on this hypothesis, many labs including ours have focused substantial attention on the cell biology of APP and the mechanisms of Abeta production, both normally and in AD. To date, molecular causes of Abeta overproduction have explained only a fraction of AD, in all cases of which Abeta accumulates excessively. Yet the nature of Abeta degradation and clearance has hardly been studied. We have chosen to direct our further experiments in this renewal to this largely unexplored topic because of compelling data generated in the current period that demonstrate a time-dependent loss of Abeta40 and 42 peptides in several cell types, particularly microglia, and implicate the thiol metalloendopeptidase, insulin degrading enzyme (IDE), as the principal mediator of this loss.
Our Specific Aims are: 1) to establish quantitatively (Km, kcat, etc.) the role of IDE (and other possible Abeta-degrading proteases) in the proteolysis of extra- and intracellular Abeta in neural and non-neural cultured cells and define where in the cell IDE contacts Abeta; 2) to assess the extent to which IDE (and other proteases identified in Aim l) is expressed and actually degrades Abeta in brain regions prone vs not prone to Abeta build-up, and whether this catabolism is altered with age or in AD in humans and APP tg mice; 3) to prove that IDE can regulate Abeta levels and deposition in vivo by creating PDGF-IDE tg mice, crossing them with PDGF-APP tg mice and assessing the progeny biochemically and pathologically; and 4) to extend our intriguing-data that IDE, besides cleaving Abeta, can mediate its conversion to stable oligomers at physiological levels. In short, we will systematically explore how Abeta is degraded extra- and intracellularly, whether IDE plays a key role in this, and how extracellular levels of Abeta monomer are regulated simultaneously by cleavage and oligomerization. Our plan utilizes the 3 complementary approaches of cell culture, in situ analyses in human and mouse brain tissues, and in vivo modelling in IDE/APP transgenic mice to decipher how Abeta proteolysis and aggregation occur under physiological conditions. The results should help open up a new area of AD pathobiology, with attendant therapeutic implications.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute on Aging (NIA)
Type
Research Project (R01)
Project #
2R01AG012749-05
Application #
2759396
Study Section
Special Emphasis Panel (ZRG1-BDCN-3 (01))
Program Officer
Oliver, Eugene J
Project Start
1995-01-01
Project End
2002-06-30
Budget Start
1999-08-01
Budget End
2000-06-30
Support Year
5
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Brigham and Women's Hospital
Department
Type
DUNS #
071723621
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Yang, Ting; Hong, Soyon; O'Malley, Tiernan et al. (2013) New ELISAs with high specificity for soluble oligomers of amyloid ?-protein detect natural A? oligomers in human brain but not CSF. Alzheimers Dement 9:99-112
Holmes, Oliver; Paturi, Swetha; Ye, Wenjuan et al. (2012) Effects of membrane lipids on the activity and processivity of purified ýý-secretase. Biochemistry 51:3565-75
Meissner, Cathrin; Lorenz, Holger; Weihofen, Andreas et al. (2011) The mitochondrial intramembrane protease PARL cleaves human Pink1 to regulate Pink1 trafficking. J Neurochem 117:856-67
Hong, Soyon; Quintero-Monzon, Omar; Ostaszewski, Beth L et al. (2011) Dynamic analysis of amyloid ?-protein in behaving mice reveals opposing changes in ISF versus parenchymal A? during age-related plaque formation. J Neurosci 31:15861-9
Wang, Xinnan; Winter, Dominic; Ashrafi, Ghazaleh et al. (2011) PINK1 and Parkin target Miro for phosphorylation and degradation to arrest mitochondrial motility. Cell 147:893-906
Sala Frigerio, Carlo; Fadeeva, Julia V; Minogue, Aedin M et al. (2010) beta-Secretase cleavage is not required for generation of the intracellular C-terminal domain of the amyloid precursor family of proteins. FEBS J 277:1503-18
Leissring, Malcolm A; Malito, Enrico; Hedouin, Sabrine et al. (2010) Designed inhibitors of insulin-degrading enzyme regulate the catabolism and activity of insulin. PLoS One 5:e10504
Espuny-Camacho, Ira; Dominguez, Diana; Merchiers, Pascal et al. (2010) Peroxisome proliferator-activated receptor gamma enhances the activity of an insulin degrading enzyme-like metalloprotease for amyloid-beta clearance. J Alzheimers Dis 20:1119-32
Cabrol, Christelle; Huzarska, Malwina A; Dinolfo, Christopher et al. (2009) Small-molecule activators of insulin-degrading enzyme discovered through high-throughput compound screening. PLoS One 4:e5274
Hemming, Matthew L; Elias, Joshua E; Gygi, Steven P et al. (2009) Identification of beta-secretase (BACE1) substrates using quantitative proteomics. PLoS One 4:e8477

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