Abstract

EXCEED THE SPACE PROVIDED. Until recently, amyloidosis was considered an obscure disease. The role of amyloid in adult-onset diabetes, and its potential contribution to Alzheimer's disease are among the factors that have stimulated much heightened ; attention to the molecular bas.es of these disorders. In addition,the physicochemical properties that cause some proteins to form amyloids are.relevant to other protein aggregation, or conformational,diseases ranging from cataracts to Parkinson's disease. While most antibody light chains show no tendency to aggregate or cause i disease, some form amyloid fibrils and others are involved in nonfibrillardeposition disease. Our work has (1) ; shown a well-defined stability threshold that separates fibrillogenic and nonfibrillogeniclight chains when tested in vitro; (2) found it possible to identify over 80% of known human amyloidogenic K! light chains by the presence of at least one mutationfrom a set of four molecular risk factors. (We believe this to be the first evidence that amyloidogenic light chains can be identifiedon the basis of primary structure.); and (3) found that certain sequence-specific peptides block fibril formation in vitro, suggesting lead compounds for eventual drugs | for clinical management of light chain amyloidosis. This proposed project will attempt to provide amolecular mechanism for light chain fibril formation.
The first Aim tests a proposed conformational change that initiates ; fibrillogenesis by using inhibitory peptides, mutational analysis and crystallography.
The second Aim extends the inferences from our highly focused study of the K4subgroup to Kl, XI, and X3subgroups by generating selected mutants that will confirm the existence of fibril stability thresholds and determining subgroup specific ; variations in this threshold. Additionally, the surfaces of interaction during fibril assembly will be mapped. The goal of improved patient care will be addressed by exploring the effectiveness of peptides as a general strategyfor development of drugs for arnyloidoses.
A third aim i s directed toward the development of a transgenic mouse model for light chain amyloidosis. Such a model will provide in vivo validationfor the significance: of the in vitro properties introduced by mutations to the development of amyloidosis. PERFORMANCE SITE ========================================Section End===========================================

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK043757-12
Application #
6888171
Study Section
Pathology A Study Section (PTHA)
Program Officer
Ketchum, Christian J
Project Start
1992-05-01
Project End
2007-04-30
Budget Start
2005-05-01
Budget End
2007-04-30
Support Year
12
Fiscal Year
2005
Total Cost
$374,714
Indirect Cost

  Institution

Name
University of Chicago
Department
Type
Organized Research Units
DUNS #
005421136
City
Chicago
State
IL
Country
United States
Zip Code
60637

  Publications

Wilton, Rosemarie; Myatt, Elizabeth A; Stevens, Fred J (2004) Analysis of protein-protein interactions by simulation of small-zone gel filtration chromatography. Methods Mol Biol 261:137-54
Gidalevitz, Tali; Biswas, Chhanda; Ding, Hua et al. (2004) Identification of the N-terminal peptide binding site of glucose-regulated protein 94. J Biol Chem 279:16543-52
Pokkuluri, P R; Gu, M; Cai, X et al. (2002) Factors contributing to decreased protein stability when aspartic acid residues are in beta-sheet regions. Protein Sci 11:1687-94
Zavaljevski, Nela; Stevens, Fred J; Reifman, Jaques (2002) Support vector machines with selective kernel scaling for protein classification and identification of key amino acid positions. Bioinformatics 18:689-96
Pokkuluri, P R; Raffen, R; Dieckman, L et al. (2002) Increasing protein stability by polar surface residues: domain-wide consequences of interactions within a loop. Biophys J 82:391-8
Davis, D P; Gallo, G; Vogen, S M et al. (2001) Both the environment and somatic mutations govern the aggregation pathway of pathogenic immunoglobulin light chain. J Mol Biol 313:1021-34
Stevens, F J (2001) Caveat receptor: proteomes on display. Comb Chem High Throughput Screen 4:599-602
Lin, Y M; Raffen, R; Zhou, Y et al. (2001) Amyloid fibril formation in microwell plates for screening of inhibitors. Amyloid 8:182-93
Stevens, F J; Kisilevsky, R (2000) Immunoglobulin light chains, glycosaminoglycans, and amyloid. Cell Mol Life Sci 57:441-9
Pokkuluri, P R; Cai, X; Johnson, G et al. (2000) Change in dimerization mode by removal of a single unsatisfied polar residue located at the interface. Protein Sci 9:1852-5

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