| Date | November 2018 | Marks available | 4 | Reference code | 18N.3.hl.TZ0.8 |
| Level | HL | Paper | 3 | Time zone | TZ0 |
| Command term | Compare and contrast | Question number | 8 | Adapted from | N/A |
Question
Enzymes are mainly globular proteins.
Describe the interaction responsible for the secondary structure of a protein.
Explain the action of an enzyme and state one of its limitations.
Contrast the actions of non-competitive and competitive inhibitors of an enzyme and state their effects on the maximum rate of reaction, Vmax, and the Michaelis–Menten constant, Km.
Markscheme
hydrogen bonding ✔
between C=O and H–N «groups» ✔
Accept a diagram which shows hydrogen bonding for M1 and which shows the interaction between O of C=O and H of NH groups for M2.
Accept “between amido/amide/carboxamide” but not “between amino/amine” for M2.
Enzyme action:
Any two of:
substrate binds to active site ✔
weakens bonds in substrate ✔
lowers activation energy
OR
provides alternate pathway ✔
increases rate of reaction
OR
acts as catalyst ✔
substrate specific ✔
Limitation:
Any one of:
temperature dependent ✔
pH dependent ✔
can be sensitive to heavy metal ions ✔
sensitive to denaturation ✔
can be inhibited ✔
substrate specific ✔
Accept “favourable orientation/conformation of the substrate «enforced by enzyme»” for M1.
Do not accept “substrate specific” as both an enzyme action and a limitation.
Award [1] for each action.
Award [1] for any two effects stated correctly.
Award [2 max] if both actions and effects are switched to incorrect inhibitor types.
Examiners report
Syllabus sections
-
17M.3.hl.TZ1.15a:
Deduce the pH range in which glycine is an effective buffer in basic solution.
-
19M.3.hl.TZ1.12a(i):
A Michaelis–Menten plot for an enzyme-catalysed reaction is shown.
Sketch a curve to show the effect of a competitive inhibitor.
-
17N.3.hl.TZ0.11a:
Determine the value of the Michaelis constant, Km, by annotating the graph.
-
17N.3.hl.TZ0.11b.i:
The malonate ion acts as an inhibitor for the enzyme.
Suggest, on the molecular level, how the malonate ion is able to inhibit the enzyme.
-
17M.3.hl.TZ1.15c:
Outline the action of a non-competitive inhibitor on the enzyme-catalysed reaction.
-
19M.3.hl.TZ2.10a(ii):
Calculate the pH of the glutamine solution using section 1 of the data booklet.
- 19N.3.hl.TZ0.11a: Outline the significance of the Michaelis constant Km.
-
19N.3.hl.TZ0.11b:
Compare the effects of competitive and non-competitive inhibitors.
-
19M.3.hl.TZ2.9c:
State and explain how a competitive inhibitor affects the maximum rate, Vmax, of an enzyme-catalyzed reaction.
-
16N.3.hl.TZ0.14b:
(i) Outline what is meant by product inhibition as it applies to hexokinase.
(ii) Product inhibition of hexokinase does not affect its Km value. Using this information, deduce the type of binding site that the inhibitor attaches to.
-
17N.3.hl.TZ0.11b.ii:
Draw a curve on the graph above showing the effect of the presence of the malonate ion inhibitor on the rate of reaction.
-
17M.3.hl.TZ2.13b:
Sketch a second graph on the same axes to show how the reaction rate varies when a competitive inhibitor is present.
-
19M.3.hl.TZ1.12a(ii):
Suggest, based on the Michaelis–Menten plot, how a competitive inhibitor such as ethanol reduces the toxicity of methanol.
-
18M.3.hl.TZ2.8d:
Calculate the pH of a buffer system with a concentration of 1.25 × 10−3 mol dm−3 carbonic acid and 2.50 × 10−2 mol dm−3 sodium hydrogen carbonate. Use section 1 of the data booklet.
pKa (carbonic acid) = 6.36
-
19N.3.hl.TZ0.10b(iii):
Calculate the ratio of [A−] : [HA] in a buffer of pH 6.0 given that pKa for the acid is 4.83, using section 1 of the data booklet.
-
18M.3.hl.TZ1.9b:
Outline the significance of the value of the Michaelis constant, Km.
-
18M.3.hl.TZ2.8g:
A different series of pepsin samples is used to develop a calibration curve.
Estimate the concentration of an unknown sample of pepsin with an absorbance of 0.30 from the graph.
-
17M.3.hl.TZ2.13a:
Determine the value of the Michaelis constant, Km, including units, from the graph.
-
17M.3.hl.TZ2.8c.ii:
Calculate the pH of a buffer solution which contains 0.700 mol dm–3 of the zwitterion and 0.500 mol dm–3 of the anionic form of alanine.
Alanine pKa = 9.87.
-
19M.3.hl.TZ2.10a(i):
Outline which pKa value should be used when calculating the pH of the solution, giving your reason.
-
17M.3.hl.TZ2.13c:
Outline the significance of the value of Km.
- 20N.3.hl.TZ0.10a: Identify the type of inhibition shown in the graph.
-
20N.3.hl.TZ0.10b(i):
Determine the value of and in the absence and presence of the inhibitor.
-
17M.3.hl.TZ1.15b:
Enzymes are biological catalysts.
The data shows the effect of substrate concentration, [S], on the rate, v, of an enzyme-catalysed reaction.
Determine the value of the Michaelis constant (Km) from the data. A graph is not required.
-
18M.3.hl.TZ2.8f:
UV-Vis spectroscopy can be used to determine the unknown concentration of a substance in a solution.
Calculate the concentration of an unknown sample of pepsin with an absorbance of 0.725 using section 1 of the data booklet.
Cell length = 1.00 cm
Molar absorptivity (extinction coefficient) of the sample = 49650 dm3 cm−1 mol−1
-
16N.3.hl.TZ0.14a:
(i) Estimate the Km values of the two enzymes.
(ii) Suggest, with a reason, which enzyme will be more responsive to changes in the concentration of glucose in the blood.
-
18M.3.hl.TZ1.9a:
Explain with reference to the binding site on the enzyme how a non-competitive inhibitor lowers the value of Vmax.
-
20N.3.hl.TZ0.10b(ii):
Outline the significance of the value of the Michaelis constant, .
-
16N.3.hl.TZ0.13c:
Amino acids act as buffers in solution. In aspartic acid, the side chain (R group) carboxyl has pKa = 4.0. Determine the percentage of the side chain carboxyl that will be ionized (–COO–) in a solution of aspartic acid with pH = 3.0. Use section 1 of the data booklet.
-
19M.3.hl.TZ1.12b:
Enzymatic activity is studied in buffered aqueous solutions.
Calculate the ratio in which 0.1 mol dm−3 NaH2PO4 (aq) and 0.1 mol dm−3 Na2HPO4 (aq) should be mixed to obtain a buffer with pH = 6.10. Use section 1 of the data booklet.
pKa (NaH2PO4) = 7.20
