Abstract

The major goal of the proposed research is to understand the molecular basis of lysosomal storage diseases, a collection of more than 40 inherited metabolic disorders that affect approximately 1 in 7,700 births. Lysosomal storage disorders are caused by defects in single genes, where the loss of a functional enzyme in the lysosome leads to accumulation of substrate and the development of disease symptoms. Lysosomal storage diseases are some of the best understood members of the larger protein-misfolding disease family, which includes Alzheimer's, Parkinson's, and Huntington's diseases. Because lysosomal storage diseases are generally caused by defects in single genes, the genetics of the diseases are simpler than in many human diseases. Lysosomal storage diseases are very active targets of clinical research, with enzyme replacement therapy, pharmacological chaperone therapy, substrate reduction therapy, bone marrow transplantation, gene therapy, and stem cell therapy approaches either approved or under clinical investigation. Despite hundreds of kilograms of recombinant enzymes produced industrially, the lack of basic knowledge about the structure, ligand binding, catalysis, and stability of the clinical targets has slowed clinical progress. For a lysosomal enzyme to function correctly, several critical steps must occur: the newly synthesized polypeptide must translocate into the Endoplasmic Reticulum (ER), where it must fold correctly; it must be post-translationally modified, allowing it to traffic through the Golgi apparatus to the lysosome; there, it must have the correct catalytic machinery and sufficient stability to perform its enzymatic task. A failure in any of these steps leads to loss of enzymatic function and subsequent disease progression. The understanding and treatment of lysosomal storage diseases has been limited by lack of understanding of the molecular defects that lead to disease symptoms. We will examine the basic biochemistry and biophysics at the root of lysosomal storage diseases, which will propel further translational progress on the diseases. To better understand the development of lysosomal storage diseases and other protein folding diseases, we propose to study the folding, stability, and function of lysosomal enzymes. We have developed methods for studying the biochemistry, biophysics, and cell biology of human lysosomal enzymes, allowing us to interrogate each stage in the maturation of the enzymes, from synthesis to trafficking to function in the lysosome. We are in the unique position to apply our expertise in the structural and cellular biology of human glycoproteins to the problem of lysosomal storage disorders. We have determined the three- dimensional structures of more human lysosomal enzymes than any other group, putting us in a unique position to study the basic biochemistry and biophysics of the family of proteins. By directly tackling difficult targets (human lysosomal enzymes are typically heavily glycosylated and otherwise post-translationally modified multimers) of high clinical significance, we advance the knowledge and treatment of disease.

Public Health Relevance

Lysosomal storage diseases are inherited metabolic diseases caused by a single defect in a single gene. We study these inherited diseases by examining the shape and stability of the proteins that are damaged in the diseases, allowing us to better understand how the diseases progress and how to better treat them.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK076877-11
Application #
9567545
Study Section
Macromolecular Structure and Function B Study Section (MSFB)
Program Officer
Eggerman, Thomas L
Project Start
2007-04-01
Project End
2022-07-31
Budget Start
2018-08-01
Budget End
2019-07-31
Support Year
11
Fiscal Year
2018
Total Cost
Indirect Cost

  Institution

Name
University of Massachusetts Amherst
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
153926712
City
Hadley
State
MA
Country
United States
Zip Code

  Publications

Germain, Dominique P; Brand, Eva; Burlina, Alessandro et al. (2018) Phenotypic characteristics of the p.Asn215Ser (p.N215S) GLA mutation in male and female patients with Fabry disease: A multicenter Fabry Registry study. Mol Genet Genomic Med :
Hingorani, Karan S; Metcalf, Matthew C; Deming, Derrick T et al. (2017) Ligand-promoted protein folding by biased kinetic partitioning. Nat Chem Biol 13:369-371
Zhou, Yan-Feng; Metcalf, Matthew C; Garman, Scott C et al. (2016) Human acid sphingomyelinase structures provide insight to molecular basis of Niemann-Pick disease. Nat Commun 7:13082
Taabazuing, Cornelius Y; Fermann, Justin; Garman, Scott et al. (2016) Substrate Promotes Productive Gas Binding in the ?-Ketoglutarate-Dependent Oxygenase FIH. Biochemistry 55:277-86
Ferreira, Susana; Auray-Blais, Christiane; Boutin, Michel et al. (2015) Variations in the GLA gene correlate with globotriaosylceramide and globotriaosylsphingosine analog levels in urine and plasma. Clin Chim Acta 447:96-104
Ferreira, Susana; Ortiz, Alberto; Germain, Dominique P et al. (2015) The alpha-galactosidase A p.Arg118Cys variant does not cause a Fabry disease phenotype: data from individual patients and family studies. Mol Genet Metab 114:248-58
Ryan, Kelly C; Guce, Abigail I; Johnson, Olivia E et al. (2015) Nickel superoxide dismutase: structural and functional roles of His1 and its H-bonding network. Biochemistry 54:1016-27
Kolli, Nilima; Garman, Scott C (2014) Proteolytic activation of human cathepsin A. J Biol Chem 289:11592-600
Molla, Mijanur Rahaman; Marcinko, Tyler; Prasad, Priyaa et al. (2014) Unlocking a caged lysosomal protein from a polymeric nanogel with a pH trigger. Biomacromolecules 15:4046-53
Mohr, Benjamin G; Dobson, Cassidy M; Garman, Scott C et al. (2013) Electrostatic origin of in vitro aggregation of human ýý-crystallin. J Chem Phys 139:121914

Showing the most recent 10 out of 21 publications