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Literature DB >> 19846563

Mutant N143P reveals how Na+ activates thrombin.

Weiling Niu¹, Zhiwei Chen¹, Leslie A Bush-Pelc¹, Alaji Bah¹, Prafull S Gandhi¹, Enrico Di Cera².

Abstract

The molecular mechanism of thrombin activation by Na(+) remains elusive. Its kinetic formulation requires extension of the classical Botts-Morales theory for the action of a modifier on an enzyme to correctly account for the contribution of the E*, E, and E:Na(+) forms. The extended scheme establishes that analysis of k(cat) unequivocally identifies allosteric transduction of Na(+) binding into enhanced catalytic activity. The thrombin mutant N143P features no Na(+)-dependent enhancement of k(cat) yet binds Na(+) with an affinity comparable to that of wild type. Crystal structures of the mutant in the presence and absence of Na(+) confirm that Pro(143) abrogates the important H-bond between the backbone N atom of residue 143 and the carbonyl O atom of Glu(192), which in turn controls the orientation of the Glu(192)-Gly(193) peptide bond and the correct architecture of the oxyanion hole. We conclude that Na(+) activates thrombin by securing the correct orientation of the Glu(192)-Gly(193) peptide bond, which is likely flipped in the absence of cation. Absolute conservation of the 143-192 H-bond in trypsin-like proteases and the importance of the oxyanion hole in protease function suggest that this mechanism of Na(+) activation is present in all Na(+)-activated trypsin-like proteases.

Entities: Chemical Gene Mutation

Mesh：

Substances：
Sodium
Thrombin

Year: 2009 PMID： 19846563 PMCID： PMC2794733 DOI： 10.1074/jbc.M109.069500

Source DB: PubMed Journal: J Biol Chem ISSN： 0021-9258 Impact factor: 5.157

101 in total

1. Thermodynamics of Na+ binding to coagulation serine proteases.

Authors: N Griffon; E Di Stasio
Journal: Biophys Chem Date: 2001-03-15 Impact factor: 2.352

2. An extensive interaction interface between thrombin and factor V is required for factor V activation.

Authors: T Myles; T H Yun; S W Hall; L L Leung
Journal: J Biol Chem Date: 2001-04-18 Impact factor: 5.157

3. Unexpected crucial role of residue 225 in serine proteases.

Authors: E R Guinto; S Caccia; T Rose; K Fütterer; G Waksman; E Di Cera
Journal: Proc Natl Acad Sci U S A Date: 1999-03-02 Impact factor: 11.205

4. Use of a fluorescence plate reader for measuring kinetic parameters with inner filter effect correction.

Authors: Y Liu; W Kati; C M Chen; R Tripathi; A Molla; W Kohlbrenner
Journal: Anal Biochem Date: 1999-02-15 Impact factor: 3.365

5. Identification of a binding site for quaternary amines in factor Xa.

Authors: D Monnaie; D Arosio; N Griffon; T Rose; A R Rezaie; E Di Cera
Journal: Biochemistry Date: 2000-05-09 Impact factor: 3.162

6. Thermodynamic linkage between the S1 site, the Na+ site, and the Ca2+ site in the protease domain of human coagulation factor xa. Studies on catalytic efficiency and inhibitor binding.

Authors: M C Underwood; D Zhong; A Mathur; T Heyduk; S P Bajaj
Journal: J Biol Chem Date: 2000-11-24 Impact factor: 5.157

7. Sodium binding site of factor Xa: role of sodium in the prothrombinase complex.

Authors: A R Rezaie; X He
Journal: Biochemistry Date: 2000-02-22 Impact factor: 3.162

8. Rational design of a potent anticoagulant thrombin.

Authors: A M Cantwell; E Di Cera
Journal: J Biol Chem Date: 2000-12-22 Impact factor: 5.157

9. Role of residue Phe225 in the cofactor-mediated, allosteric regulation of the serine protease coagulation factor VIIa.

Authors: R J Petrovan; W Ruf
Journal: Biochemistry Date: 2000-11-28 Impact factor: 3.162

10. Prothrombin Scranton: substitution of an amino acid residue involved in the binding of Na+ (LYS-556 to THR) leads to dysprothrombinemia.

Authors: W Y Sun; D Smirnow; M L Jenkins; S J Degen
Journal: Thromb Haemost Date: 2001-04 Impact factor: 5.249

17 in total

Mutant N143P reveals how Na+ activates thrombin.

1. Thermodynamics of Na+ binding to coagulation serine proteases.

2. An extensive interaction interface between thrombin and factor V is required for factor V activation.

3. Unexpected crucial role of residue 225 in serine proteases.

4. Use of a fluorescence plate reader for measuring kinetic parameters with inner filter effect correction.

5. Identification of a binding site for quaternary amines in factor Xa.

6. Thermodynamic linkage between the S1 site, the Na+ site, and the Ca2+ site in the protease domain of human coagulation factor xa. Studies on catalytic efficiency and inhibitor binding.

7. Sodium binding site of factor Xa: role of sodium in the prothrombinase complex.

8. Rational design of a potent anticoagulant thrombin.

9. Role of residue Phe225 in the cofactor-mediated, allosteric regulation of the serine protease coagulation factor VIIa.

10. Prothrombin Scranton: substitution of an amino acid residue involved in the binding of Na+ (LYS-556 to THR) leads to dysprothrombinemia.

Review 1. Conformational selection in trypsin-like proteases.

2. Crystal structure of thrombin bound to the uncleaved extracellular fragment of PAR1.

3. Why Ser and not Thr brokers catalysis in the trypsin fold.

4. Crystal structure of prethrombin-1.

5. Redesigning allosteric activation in an enzyme.

Review 6. Allostery in trypsin-like proteases suggests new therapeutic strategies.

Review 7. Biomolecular electrostatics and solvation: a computational perspective.

8. A revisit to the one form kinetic model of prothrombinase.

Review 9. Molecular Mechanisms of Enzyme Activation by Monovalent Cations.

10. Loop Electrostatics Asymmetry Modulates the Preexisting Conformational Equilibrium in Thrombin.