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Hypothetical substrate docking in enzyme’s active site . Substrate is geometrically and electronically compatible with active site. Enzymes are also stereospecific. ES complex formation. How is G ‡ lowered?.
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Hypothetical substrate docking in enzyme’s active site. Substrate is geometrically and electronically compatible with active site. Enzymes are also stereospecific.
How is G‡ lowered? Many enzymes stabilize the transition state in addition to the mechanisms described below through relatively tight binding. Mechanisms of catalysis 1. Acid-Base catalysis 2. Covalent catalysis 3. Metal ion catalysis 4. Proximity and orientation effects 5. Electrostatic catalysis
Acid catalysis 1. Acid-Base catalysis (H+ transfer between E and S)
2. Covalent catalysis (covalent bond between E and S) Amine in enzyme reacts with carbonyl group to form Schiff base Elimination of CO2 then does not lead to an unstable transition state
Schiff base breaks down to amine catalyst and acetone 3. Metal ion catalysis (metal ions can mediate redox reactions or electrostatically promote reactions).
Proximity/Orientation No catalyst: slow b/c few encounters Catalyst: faster
5. Electrostatic catalysis Most substrate molecules have a hydration shell that must be removed to allow reaction. Enzyme active sites are often non-aqueous (not necessarily non-polar) and they require that water is removed from the substrate before binding can occur. The non-aqueous active site allows stronger electrostatic interactions.
Chymotrypsin. 241 amino acid protein with 2 domains and an active site with 3 residues important for catalysis shown in red (His 57, Asp 102 and Ser 195). Chymotrypsin Digestive enzyme synthesized in pancreas and secreted to small intestine. Has broader specificity than most enzymes. Hydrolyzes the peptide bond following large nonpolar residues like Phenylalanine, Tryptophan or Tyrosine. Leu-Ala-Tyr-Ile-Asp
His 57 Asp 102 Ser 195 Chymotrypsin is part of a class of enzymes known as Serine Proteases. Uses acid-base and covalent catalysis, and it stabilizes the transition state.
Let’s look at the detailed reaction mechanism for chymotrypsin, a protease: It hydrolyzes peptide bonds immediately C-terminal to aromatic amino acids With a rate enhancement of > 109 And illustrates several principles Transition state stabilization Acid-base catalysis Covalent catalysis A two-phase reaction Leu-Ala-Tyr-Ile-Asp
Mechanism in the Substrate Pocket • Phase I - acylation of Ser195 • Phase 2 – deacylation of Ser195 • Follow the roles of the “catalytic triad” through the reaction: Ser195,His57 and Asp102 • What is the role of Gly193?
In the active site of chymotrypsin, know the chemical roles of: • Histidine 57 • Aspartate 102 • Serine 195 • Glycine 193
Chymotrypsin Catalytic Mechanism A1 H H C C [NH2] [HOOC] C N H C N C N C C O Catalytic Triad His57 Asp102 Ser195 O Check substrate specificity
Chymotrypsin Catalytic Mechanism A2 C C [NH2] [HOOC] C N H C N C N C C O His57 Asp102 Ser195 H H O First Transition State
Chymotrypsin Catalytic Mechanism A3 C C [NH2] [HOOC] C N H C N C N C C O H O H Acyl-Enzyme Intermediate
Chymotrypsin Catalytic Mechanism D1 C C [NH2] [HOOC] C N-H H C N C N C C O O H H H O Acyl-Enzyme Water Intermediate
Chymotrypsin Catalytic Mechanism D2 C C [NH2] C N C C O O H H H O Second Transition State
Chymotrypsin Catalytic Mechanism D3 H C C [NH2] C N C C O O H H O Deacylation