| Literature DB >> 22923379 |
Adrianne M C Pittman1, Melissa D Lage, Vladimir Poltoratsky, Justin D Vrana, Alessandro Paiardini, Alessandro Roncador, Barbara Cellini, Robert M Hughes, Chandra L Tucker.
Abstract
Many human diseases are caused by genetic mutations that decrease protein stability. Such mutations may not specifically affect an active site, but can alter protein folding, abundance, or localization. Here we describe a high-throughput cell-based stability assay, IDESA (intra-DHFR enzyme stability assay), where stability is coupled to cell proliferation in the model yeast, Saccharomyces cerevisiae. The assay requires no prior knowledge of a protein's structure or activity, allowing the assessment of stability of proteins that have unknown or difficult to characterize activities, and we demonstrate use with a range of disease-relevant targets, including human alanine:glyoxylate aminotransferase (AGT), superoxide dismutase (SOD-1), DJ-1, p53, and SMN1. The assay can be carried out on hundreds of disease alleles in parallel or used to identify stabilizing small molecules (pharmacological chaperones) for unstable alleles. As demonstration of the general utility of this assay, we analyze stability of disease alleles of AGT, deficiency of which results in the kidney stone disease, primary hyperoxaluria type I, identifying mutations that specifically affect the protein-active site chemistry.Entities:
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Year: 2012 PMID: 22923379 PMCID: PMC3522161 DOI: 10.1534/genetics.112.143750
Source DB: PubMed Journal: Genetics ISSN: 0016-6731 Impact factor: 4.562