Garman lab: Interconversion of lysosomal enzyme specificities
From Proteopedia
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(use the buttons above to compare with α-NAGAL) | (use the buttons above to compare with α-NAGAL) | ||
| + | ===Figure Y (bonus figure)=== | ||
| + | The shape of the active site is often complementary to the molecule it binds to (lock-and-key concept). This figure shows the contacts between bound molecules and active site residues. Contacts are shown as the overlap of Van der Waals spheres around atoms. Slight overlap is shown in yellow while larger overlap is shown in red. When two functional groups form a hydrogen bond, atoms come closer than they would if they interact via Van der Waals interactions, so you expect to see red overlap for hydrogen bonds. | ||
| + | Here are the contacts for α-GAL bound to galactose and α-NAGAL bound to N-acetyl galactosamine. These are observed structures, so the contacts seen explain why they bind to their ligands. | ||
| + | In contrast, here are the contacts for two hypothetical models, galactose bound to the α-NAGAL active site and N-acetyl galactosamine bound to the α-GAL active site. There are less contacts in the hypothetical α-NAGAL: galactose complex and severe clashes in the <scene name='78/786673/Clash_nagal/2'>hypothetical α-GAL: N-acetyl galactosamine complex</scene>. In fact, experiments show that α-NAGAL does bind galactose (though much more weakly than N-acetyl galactosamine) while α-GAL does not bind N-acetyl galactosamine. | ||
===Figure 2: Structure of αGAL(SA)=== | ===Figure 2: Structure of αGAL(SA)=== | ||
Revision as of 13:08, 23 July 2018
Contents |
How this page was created
The goal of this page is to provide three-dimensional and interactive figures to explore the structures determined for the 2010 paper "Interconversion of the Specificities of Human Lysosomal Enzymes Associated with Fabry and Schindler Diseases" by Ivan B. Tomasic, Matthew C. Metcalf, Abigail I. Guce, Nathaniel E. Clark and Scott C. Garman [1]. The starting point are the figures found in this paper. Biochemistry students at Westfield State University recreated these figures in jmol, and revised them after getting feedback from the authors. A special thank you goes to Susan Al Mahrwuth, Samuel J. Butler, Susy Civil, Westin G. Cohen, Allison F. DeVivo, Tyler S. Fassett, Courtney M. Fisher, Kimberly Garcia, Stephanie L. Hardy, Maureen W. Kamau, Sienna R. Kardel, Allyson L. Kress, Julia M. Lahaie, Stephen A. Malerba, Brittany E. Ricci, Kimberly Rosario, Yelena Vynar, and Deanna N. Womack for creating the initial figures and captions. If you are interested to learn how these figures were made, take a look at the discussion page (2nd tab above).
Lysosomal storage disease
Lysosomal storage disorders are inherited metabolic diseases characterized by an accumulation of undigested various toxic materials. There are nearly 50 diseases and the two examples shown here are Fabry and Schindler disease. Fabry disease, which occurs between early childhood and adolescence, is characterized by the lack of the enzyme alpha galactosidase (α-Gal). Schindler disease can occur in infancy or in adulthood and is characterized by the lack on the enzyme alpha N-acetylgalactosaminidase (α-NaGal). There are currently no cures for lysosomal storage disorders however enzyme replacement therapy is a treatment option. The basic principle of enzyme replacement therapy is to over express the enzyme of interest heterologously, in this case α-Gal α-NaGal, in a cell line and to isolate and purify it from the culture. In enzyme replacement therapy, patients are injected with the enzymes that they lack in the hopes of restoring the enzymatic activity in their cells.
Immune Response
Individuals suffering from Fabry disease cannot produce the α-GAL protein that is necessary for breaking down Galactose. The usual treatment for this is giving the patient doses of the protein, but this poses a problem. Since the body does not produce the protein, an immune response ranging from severe anaphylaxis to mild discomfort can occur when the patient is given the protein. The body does however produce α-NAGAL, a protein with a similar active site and function as Alpha Gal. Altering the active site of α-NAGAL to match that of α-GAL allows doctors to administer a protein that serves the function of Alpha Gal but has the antigenicity of α-NAGAL, which means the body will recognize the protein and not elicit an immune response.
Enzymatic activity
α-Gal and α-NaGal have relatively identical active sites, which are conserved with the exception of alanine, serine, glutamate and leucine which are positioned differently. The two enzymes have the same folds and both function by cleaving glycosydic bonds however have different substrate specificities. The differences in substrate specificity occur because α-NaGal has a larger binding pocket thus interacting with larger molecules but smaller residues.
Galactose vs. N-acetyl-galactosamine
Structures shown on this page
3H54: the enyme α-NAGAL in complex with the sugar GalNAc
3HG5: the enyme α-GAL in complex with the sugar galactose
3LX9: the enyme α-GAL(SA) in complex with the sugar GalNAc
3LXA: the enyme α-GAL(SA) in complex with the sugar galactose
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