Receptors (L5-8)

Question 1

What do most drugs target?

Answer 1

Proteins like receptors, enzymes and transporters like carriers or channels

Question 2

What is the difference between a receptor and drug target?

Answer 2

Receptors are proteins who’s function is to recognise and respond to endogenous chemical signals. Drug targets are other macromolecules which drugs interact with to produce the effect.

Question 3

What are the different types of receptor families?

Answer 3

Type 1 - ligand gated ion channels (ionotropic receptors)- they have 4/5 transmembrane spanning domains. They’re activated by ligands
Type 2 - G protein coupled receptors (metabotropic because they use energy) Have multiple binding domains with a G-protein coupled domain.
Type 3 - Kinase-linked receptors. Have a binding domain on each terminal. Binding of an extracelllar ligand causes enzymatic activity on the IC side (catalytic domain)
Type 4 - Nuclear receptors - found in the cytosol until a ligand binds then they move into the nucleus - ussually have DNA binding domains (zinc fingers)

Question 4

What does the activation of a receptor depend on?

Answer 4

The activation of a receptor by the agonist depends on the efficacy of the drug. A higher efficacy elicits a larger response.

Question 5

What what is meant by the occupancy of a receptor and what does it depend on?

Answer 5

The proportion of receptors occupied which varies with concentration. (the number of receptors occupied / total number of receptors) The affinity of the drug to the receptor - the higher the affinity, the higher the occupancy will be. Its a ratio so varies between 0 (none occupied) and 1 (all occupied)

Question 6

How can you measure the occupancy?

Answer 6

Using a tagged agonist - one with GFP on it which fluoresces when its bound to a receptor and then you can measure the amount of florescence. A higher result = a higher occupancy.

Question 7

Explain non-specific binding of ligands

Answer 7

Most ligands bind non-specifically to other things like filter paper, and glass. his can be reduced using anti-absorbants e.g. albumin or collagen for peptides or o-catechol for catecholamines. But this does not reduce non-specific binding to the tissue under study. Measuring proportions of specific and non-specific binding is a key element to an assay. Rinsing only removes unbound radio ligand (the marker) from the incubation medium.

Question 8

Explain the properties a radio ligand must have to make it useful for experiments

Answer 8

Must be biologically active because its binding is suppossed to correlate with a pharmacological action. The ligand must be extrememly pure chemically and not degrade - you can get around this by using a free radical scavenger e.g. ethanol in you drug solution. Stroing it at low temps and out of direct sunlight, and incorporating an antioxidant e.g. ascorbic acid aslo helps with this.
Labelling of the drug with readioactivity must achieve a very high specific activity ( activity per unit mas) to all very low tracer concentrations.

Question 9

What are the different radio labels that could be used to study a drug?

Answer 9

3H - Labelled product is indistinguishable from the native compund, highe specific activity can be obtained. It has a good stability when stored properly and has a long half life (12.5 yrs). However, it is expensive and difficult to use.
125I - Used if the compound has an aromatic hydroxyl group (e.g. tyrosines of peptides). It can be incoprporated at very high specific activities but the biological activity of the ligand may be reduced and it have a musch shorter half life (67 days)

Question 10

How can you separate the bound ligand from the free ligand in the incubation media?

Answer 10

by centrifugation then filtration is the ligand is insoluble. For soluble ligands (and solubilised receptors) you have to use other techniques like dialysis, column chromatography and precipitation/adsorption
The main problem is the rate of dissociation of the ligand-receptor complexes must be compatible with the affinity of a ligand for a receptor. A lower affinity (Higher KD) requires a faster, more efficient separation.

Question 11

What is a scatchard plot?

Answer 11

The plot of the ratio of the concentrations of a bound ligand to an unbound ligand. It is a method for analysing data freely for reversible ligand/receptor binding interactions where you can’t use a tagged ligand because it doesn’t stay put - help you work out the affinity constant
Specific binding =total bound - non-specific binding. It shows a plateau for specific binding because the receptors become saturated, but not for non-specific because the receptor can continue to bind to other things like the glass and tissue.
Data is plotted on a semi log scale ( The conc of the ligand is on a log scale) as this converst the retangular hyperbola into a sigmoid curve

Question 12

What is the scatchard equation?

Answer 12

B/F (specifically bound/free ligand) = Bmax (max no. of binding sites)- B / Kd (eq.binding constant) - so basically ratio of no. of receptors occupied to ligand added = total no. of receptors - specifially bound divided by dissociation constant - give you a measure of affinity

Question 13

How do you use the scatchard plot to work out the affinity constant?

Answer 13

B/F is what is plotted on the Y axis (bound radio ligand/free radioligand(approx the conc of the free ligand added in mol/litre bc the amount that ia actually bound and not free is negligible) Bmax is the max amount of drug which can bind specifically to the receptors in the preparation (also indicates the conc of receptors in the tissue) Bmax is the X intercept bc B/F = 0 when all the receptor is bound. Therefore, the slope is the inverse of - Kd (Kd is found using saturation analysis, it is the conc of the ligand which at equilibrium occupies 50% of the receptor

Question 14

How does Kd shift on an conc Vs occupancy graph?

Answer 14

A lower Kd is more the the left because the drug has a higher affinity and therefore needs less conc for a high occupancy. A high Kd means a lower affinity because a high conc is needed for the same occupancy.

Question 15

How can you use binding data to learn about the selectivity of different ligands?

Answer 15

If you try the same drug on 2 different tissues, you will see a different occupancy for each. (One will show a lower affinity). Whereas a non-selective ligand will have the same occupancy in both tissues.

Question 16

What is the EC50 of a drug?

Answer 16

the effective concentration which gives 50% of the maximal response. Therefore, it is a measure of an agonist’s potency.

Question 17

What does it mean when the graph of the EC50 and Kd are different?

Answer 17

The Ec50 curve for concentration and Kd curve for binding show similar sigmoidal curves. When they’re nor exactly the same, you an see ‘receptor reserve’ which is when not 100% of the occupied to give 100% of the response. This suggests there is amplification of the signal. Sometimes tissues can get a maximal response with less that 5% occupancy just because the signal is amplified so much.

Question 18

Explain how concentration/effect curves can be used to show potency.

Answer 18

Response = max conc of the agonist^hillslope /conc of agonist^hill slope + Conc at EC50 ^hill slope
A shift to the left by the curve means the agonist is increasing in potency because less conc is needed for a large response.
The potency of an agonist depends on affinity, efficacy and spare receptors
Agonists with different efficacies produce different maximal response curves even if they have the same EC50 due to different affinities.

Question 19

How can you tell a partial agonist?

Answer 19

If they don’t produce a maximal response as high as a full agonist even at the same concentration or higher. For a partial agonist, The EC50 = Kd

Question 20

What 3 properties determine the effect of a drug in a living system?

Answer 20

Its specificity - Interaction with structurally defined site/receptor via chemical properties or structure
affinity - the ability of an agonist/antagonist to bind to a receptor
Efficacy - The ability to activate a receptor (between 0 and 1) (antagonists have an efficacy of 0)
The affinity of a competitive antagonist for a receptor is constant. Antagonist affinity is commonly used to identify and classify receptors because it marks them and shows binding but doesn’t change them.

Question 21

What is chemical antagonism?

Answer 21

When substances combine in solution so that the effect o the active drug is lost (the agonist is chemically altered by the antagonist) e.g. inactivation of heavy metals (mercury and lead) whose toxicity is reduced with the addition of a chelating agent (dimercaprol)

Question 22

What is pharmokinetic antagonism?

Answer 22

Reduction in the amount of drug absorbed. E.g. decreases absorption from the GI tract like drugs that inhibit gut motility (opiates will reduce absorption by oral route). Can also be a change in drug metabolism. E.g. if patients are taking warfarin (antii-coagulant) you have to be careful when giving them antibiotics because they will stimulate the metabolism of Warfarin and reduce its effects

Question 23

What is physiological antagonism?

Answer 23

The interaction of 2 drugs with opposing action in the body E.g. NA raises arterial BP while histamine lowers it - so the 2 chemicals are doing opposing things, but acting through different mechanisms.

Question 24

What is non-competitive antagonism?

Answer 24

Blocks some step in the process between receptor activation and response i.e. it does not compete with the agonist for the site, it binds to a different area which stops the agonist from binding or lets it bind but stops its effect

Question 25

What is competitive antagonism?

Answer 25

Competitive antagonists compete with the agonist for the occupancy of the receptor. The one which is at the highest conc/higher affinity usually wins. Can be reversible or irreversible. Reversible e.g. effects of atropine on response to ACh for ileum shows a parallel rightward shift in conc-response curve but there is no change in the maximum response. So this shows the antagonist being present means you need a higher conc. of the agonist to produce the maximal response

Question 26

What is the dose ratio and how is it calculated?

Answer 26

Dose ratio = how many more times agonist is needed in the presence of an antagonist (conc of agonist in presence of antagonist / conc of agonists in absence of antagonist) or conc of antagonist +1 / Kd (agonist dissociation constant)

Question 27

What is a Schild analysis?

Answer 27

Used to measure antagonist affinity. log10(dose raio -1) = 0 at the X intercept, pA2 is minus this value.
pA2 =-log10 (the molar conc of the antagonist that gives a dose ratio of 2)

Question 28

Explain irreversible competitive antagonists

Answer 28

Antagonism that cannot be reverse by washing the tissue, so the drug doesnt just block the receptor, it structurally changes the receptor so the agonist can’t even bind in the absence of the antagonist. Irreversible antagonism is time dependant. E.g. the effect of alkylating drug dibenamine (1nM) on histamine responses in guinea pig ileum causes a decreases over time - the longer the antagonist is left on the tissue, the less of a response that is elicited when it is washed off.

Question 29

What is tachyphylaxis?

Answer 29

A diminishing response to successive doses of a drug, rendering it less effective. The effect is common with drugs acting on the nervous system. This desensitisation can be caused by a loss of receptor from the surface e.g. due to internalisation followed by degradation or recycling. OR it can be due o a change in the receptor itself, e.g. phosphorylation which leads to decreased coupling of receptor to effector. Can also be due to the exhaustion of mediators or an increased metabolic degradation/extrusion of the drug.