Cavitation as a Mechanism of Substrate Discrimination by Adenylosuccinate Synthetases
Abstract
Adenylosuccinate synthetase catalyzes the first committed step in the de novo biosynthesis of AMP, coupling l-aspartate and IMP to form adenylosuccinate. Km values of IMP and 2'-deoxy-IMP are nearly identical with each substrate supporting comparable maximal velocities. Nonetheless, the Km value for l-aspartate and the Ki value for hadacidin (a competitive inhibitor with respect to l-aspartate) are 29−57-fold lower in the presence of IMP than in the presence of 2'-deoxy-IMP. Crystal structures of the synthetase ligated with hadacidin, GDP, and either 6-phosphoryl-IMP or 2'-deoxy-6-phosphoryl-IMP are identical except for the presence of a cavity normally occupied by the 2'-hydroxyl group of IMP. In the presence of 6-phosphoryl-IMP and GDP (hadacidin absent), the l-aspartate pocket can retain its fully ligated conformation, forming hydrogen bonds between the 2'-hydroxyl group of IMP and sequence-invariant residues. In the presence of 2'-deoxy-6-phosphoryl-IMP and GDP, however, the l-aspartate pocket is poorly ordered. The absence of the 2'-hydroxyl group of the deoxyribonucleotide may destabilize binding of the ligand to the l-aspartate pocket by disrupting hydrogen bonds that maintain a favorable protein conformation and by the introduction of a cavity into the fully ligated active site. At an approximate energy cost of 2.2 kcal/mol, the unfavorable thermodynamics of cavity formation may be the major factor in destabilizing ligands at the l-aspartate pocket.
Additional Information
© 2006 American Chemical Society. Received 18 April 2006. Published online 2 September 2006. Published in print 1 September 2006. This work was supported by National Institutes of Health Grant NS 10546.Additional details
- Eprint ID
- 73897
- Resolver ID
- CaltechAUTHORS:20170131-140942966
- NS 10546
- NIH
- Created
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2017-02-01Created from EPrint's datestamp field
- Updated
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2021-11-11Created from EPrint's last_modified field