L19: Fundamental Enzyme Kinetics Flashcards
[ES]
Determination of [ES] is difficult or impossible
Fairly constant over much of reaction i.e. reaction is in steady state
Vmax
Velocity of reaction at saturating substrate
Km
Substrate required to give velocity of vmax/2
True measure of affinity of enzyme for its substrate
Reversible enzyme inhibition: competitive inhibition
Inhibitor competes with substrate for same binding site on enzyme
At high substrate conc -> substrate outcompetes inhibitor -> no inhibition
-> Vmax achieved at infinite substrate conc, is not affected by inhibitor
More substrate required to achieve half Vmax -> apprent Km larger than presence of inhibitor
Lineweaver-burk: intersecting lines, intersection on 1/v axis
Uncompetitive inhibition
Inhibitor can only bind enzyme-substrate complex and not to the free enzyme
Binding of substrate to enzyme to form ES -> binding site for inhibitor at active site or induces conformational change in enzyme -> creates remote binding site for inhibitor
Enzyme-substrate-inhibitor complex unable to catalyse formation of product from substrate
Even at high substrate conc inhibition occurs -> Vmax reduced
As inhibitor binds to ES-> equilibrium between E & ES in favour of ES -> Km (Kmapp) is smaller in presence of inhibitor
Lineweaver-burk: parallel lines
Mixed or noncompetitive
Inhibitor binds to enzyme and ES
Inhibitor may bind more tightly to E than ES -> KI > KIS or the opp. If bound equally well (KI=KIS) -> noncompetitive
Vmax decreased in presence of inhibitor (uncompetitive component)
Competitive dominates (KI Km will increase in presence of inhibitor
Uncompetitive dominates (KIS Kmapp decreased in presence of inhibitor
If neither dominate (KI=KIS) -> Kmapp unaffected by the presence of inhibitor -> =Km
Lineweaver-burk: intersecting lines which intersect to left of 1/v axis
Irreversible enzymes inhibition
Involves irreversible formation of covalent bond between inhibitor and enzyme, usually at active site
Usually time dependent and loss of enzyme activity can be monitored
Example of irreversible enzyme inhibition
Penicillin: irreversible inhibitor of glycopeptidyl transpeptidase (essential for bacterial cell wall synthesis). A suicide substrate (similar structure to normal substrate -> binds with high affinity to enzyme
Ser-OH in enzyme attacks carbonyl carbon in penicillin as if it were a peptide bond in protein
Once bond between Ser and carbon formed -> cant be broken
Allosteric enzyme
Important regulators of metabolism
Regulated by its substrate and activators and inhibitors
Multi-subunit proteins (have quarternary structure). Subunits exist in 2 different structural conformations: T state and R state which are in equilibrium
T state
Binds substrate with low affinity
Absence of substrate -> most of subunits in T state -> Km for substrate is high (low affinity)
Allosteric inhibitor -> shifts equilibrium in favour of T -> plot of v vs [subs] even more sigmoidal. At most [subs], v will be lower than in absence of inhibitor
R state
Substrate increase -> more substrate binds to enzyme -> equilibrium between T & R states shifted in favour of R state -> Km decreases
At saturating substrate conc all enzyme in R state
Allosteric activator -> shift equilibrium in favour of R
If sufficient activator present -> all of enzyme will be in R state -> plot of v vs [subs] in normal hyperbolic form (Km remains constant and at most [subs], v will be higher than in absence of activator)
Michaelis-menten equation
V= Vmax[S]/Km + [S]
Vmax/(1+Km/[S])
