The Equilibrium Binding Constant and Binding Strength of Proteins - Concept | Molecular Biology | JoVe

In the cell, proteins randomly collide with other molecules, such as other proteins, nucleic acids, and small-molecule ligands.

If the binding is non-specific, few non-covalent interactions between the molecules result in a brief association.

If a specific ligand binds to the protein, it forms extensive non-covalent interactions along complementary surfaces. Such complexes are stable, staying bound for a long time, before dissociating.

The strength of a binding interaction is reported in terms of its equilibrium constant, K_b, also called the binding or association constant.

K_b can be calculated from the ratio of the concentration of protein-ligand complex over the concentrations of unbound protein and ligand found at equilibrium.

Given its relation with the free energy change due to binding, a large K_b means a large decrease in delta G, indicating strong affinity between protein and ligand.

Two competing processes are important for protein-ligand binding: the association of a protein and a ligand to form a complex and the dissociation of the complex into the reactants.

The association constant, k_on, is a measure of the number of binding events per second between a protein and its ligand; it can be used to calculate the rate of ligand binding to the protein at a given concentration.

Conversely, k_off, is a measure of the number of dissociation events; it can be used to calculate how quickly the complex comes apart.

When the rate of association equals the rate of dissociation, an equilibrium is reached, where the net concentrations of products and reactants remain constant.

Thus, at equilibrium, k_on times the product of the equilibrium concentrations of the protein and the ligand equals k_off times the equilibrium concentration of the protein-ligand complex.

Rearranging this expression also shows that the ratio of k_on to k_off equals K_b at equilibrium.

The equilibrium binding constant (K_b) quantifies the strength of a protein-ligand interaction. K_bcan be calculated as follows when the reaction is at equilibrium:

Eq1

where P and L are the unbound protein and ligand, respectively, and PL is the protein-ligand complex.

As the amount of bound ligand is also related to the rate of ligand binding, experiments can also determine K_b by examining the rates of protein-ligand association (k_on) and dissociation (k_off) using the following ratio:

Eq1

Thus, two categories of binding assays are used to determine the equilibrium binding constant – those that measure equilibrium concentrations and those that measure a reaction’s kinetics. In case, the reaction must be at equilibrium at the time of measurement.

The method of determining the equilibrium concentrations depends on the desired sensitivity and ease of signal detection. For these reasons, spectroscopic assays are most widely used. In these experiments, the reaction produces an absorbance change of a reactant or a product at a given wavelength, detectable by a UV-Vis spectrophotometer. Alternatively, the reactant or product can be tagged with a fluorescent probe or may contain an intrinsic fluorophore. Then, the reaction progress can be measured from the change in fluorescence. These assays are performed by varying one reactant’s concentrations while the rest of the experiment is held constant. The results can then be graphed and analyzed with various curve fitting methods.

Interactions between proteins and ligands are also studied using a variety of biochemical and spectroscopic techniques. Structural analysis, using X-ray crystallography and NMR spectroscopy, aids in predicting protein-ligand interactions through molecular simulations. Theoretical and computational approaches, such as protein-ligand docking studies, are used extensively to characterize the position and interactions of small molecule ligands, including drug candidates. Computer-aided drug design is a fast and low-cost alternative to accelerate the pace of conventional trial and error drug testing.

Tags

Equilibrium Binding Constant Binding Strength Non specific Binding Specific Ligand Binding Non covalent Interactions Stable Complexes Dissociation Concentration Ratio Affinity Association Constant Kon Ligand Binding Rate Dissociation Constant Koff

Aus Kapitel 4:

article

Now Playing

4.4 : Die Gleichgewichts-Bindungskonstante und die Bindungsstärke

Protein Function

12.7K Ansichten

article

4.1 : Ligandenbindungsstellen

Protein Function

12.6K Ansichten

article

4.2 : Protein-Protein-Schnittstellen

Protein Function

12.4K Ansichten

article

4.3 : Konservierte Bindungsstellen

Protein Function

4.1K Ansichten

article

4.5 : Cofaktoren und Coenzyme

Protein Function

7.2K Ansichten

article

4.6 : Allosterische Regulation

Protein Function

13.9K Ansichten

article

4.7 : Ligandenbindung und -verknüpfung

Protein Function

4.7K Ansichten

article

4.8 : Kooperative allosterische Übergänge

Protein Function

7.8K Ansichten

article

4.9 : Phosphorylierung

Protein Function

5.8K Ansichten

article

4.10 : Proteinkinasen und Phosphatasen

Protein Function

12.9K Ansichten

article

4.11 : GTPasen und deren Regulation

Protein Function

8.1K Ansichten

article

4.12 : Kovalent gebunden Protein-Regulatoren

Protein Function

6.6K Ansichten

article

4.13 : Proteinkomplexe mit austauschbaren Komponenten

Protein Function

2.5K Ansichten

article

4.14 : Mechanische Proteinfunktionen

Protein Function

4.9K Ansichten

article

4.15 : Strukturelle Proteinfunktionen

Protein Function

27.1K Ansichten

See More

Copyright © 2025 MyJoVE Corporation. Alle Rechte vorbehalten