
A key feature of factor IXa is its allosteric transformation from an enzymatically latent form into a potent procoagulant. Although several small molecules have been found to be capable of partially affecting FIXa function (i.e. ethylene glycol, Ca(2+), and low molecular weight heparin [LMWH]), the resulting modest changes in peptidolytic activity have made the study of their mechanisms of action challenging. As these effects provide hints about potential regulatory forces that may be operational in the full expression of FIXa coagulant activity, their description remains of great interest. Studies of crystal structures have yielded insights into the structural changes induced by these effectors, but there remains a paucity of information to correlate any given structural change with specific consequences for FIXa function.To correlate structural changes induced by these modulators with defined consequences for FIXa substrate discrimination and function.A peptidomics-based mass spectrometry (MS) approach was used to examine the patterns of hydrolysis of four combinatorial chemistry-derived pentapeptide libraries by FIXa under various conditions in a soluble, active enzyme system.Ethylene glycol specifically altered the S3 subsite of FIXa to render it more tolerant to side chains at the P3 substrate position, whereas Ca(2+) enhanced tolerance at the S2 subsite. In contrast, LMWH altered both the S2 and S1' subsites.These results demonstrate the role of plasticity in regulating FIXa function with respect to discrimination of extended substrate sequences, as well as providing crucial insights into active site modulations that may be capitalized on by various physiologic cofactors of FIXa and in future drug design.
Models, Molecular, Proteomics, Ethylene Glycol, Protein Conformation, blood clotting factor 9a, ethylene glycol, peptide library, Factor IXa, Substrate Specificity, Structure-Activity Relationship, Models, Peptide Library, Catalytic Domain, calcium ion, Matrix-Assisted Laser Desorption-Ionization, Combinatorial Chemistry Techniques, Humans, Hemophilia, Molecular Biology, mass spectrometry, Binding Sites, Heparin, Spectrometry, low molecular weight heparin, Hydrolysis, article, peptidomics, Low-Molecular-Weight, Structure, Molecular, Thrombosis, molecular docking, Mass, Heparin, Low-Molecular-Weight, enzyme activity, Kinetics, hydrolysis, priority journal, Chromogenic Compounds, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Enzymology, Calcium, Peptidomimetics, Substrate, Oligopeptides, combinatorial chemistry
Models, Molecular, Proteomics, Ethylene Glycol, Protein Conformation, blood clotting factor 9a, ethylene glycol, peptide library, Factor IXa, Substrate Specificity, Structure-Activity Relationship, Models, Peptide Library, Catalytic Domain, calcium ion, Matrix-Assisted Laser Desorption-Ionization, Combinatorial Chemistry Techniques, Humans, Hemophilia, Molecular Biology, mass spectrometry, Binding Sites, Heparin, Spectrometry, low molecular weight heparin, Hydrolysis, article, peptidomics, Low-Molecular-Weight, Structure, Molecular, Thrombosis, molecular docking, Mass, Heparin, Low-Molecular-Weight, enzyme activity, Kinetics, hydrolysis, priority journal, Chromogenic Compounds, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Enzymology, Calcium, Peptidomimetics, Substrate, Oligopeptides, combinatorial chemistry
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