Michaelis-Menten kinetics
For an enyzme reaction that obeys Michaelis-Menten kinetics:
- S: solute concentration
- V0: initial rate (velocity) of reaction
- VMAX: the maximum rate of reaction when all enzyme active sites are saturated with substrate velocity
- Km (Michaelis constant): the substrate concentration that gives half maximal velocity
- Km = [S] at 0.5(VMAX)
- Low Km = enzyme only needs a small amount of substrate to work at half max velocity (+ reverse)
Calculating Km
- Km = (k-1+k2)k1
- k1 = forward rate for enzyme association with substrate
- k-1 = backwards rate for enzyme dissociation with substrate
- k2 = forward rate of enzyme conversion from energy to product
Lineweaver-Burk Plot
- VMAX = intersection of line with Y axis
- KM = intersection of line with X axis
Enzyme inhibition
Reversible inhibition
Competitive
- Binds to active site
- VMAX stays the same
- Km varies
Non-competitive
- Binds to allosteric site
- Km stays the same
- VMAX varies
Irreversible inhibition
- Non-competitive - usually involves formation/breakage of covalent bonds in the enzyme complex
Enzyme regulation
- Allosteric control - inhibition of rate limiting enzymes by end products
- Sigmoidal curve
- Example: binding of oxygen to haemoglobin
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