Simulation of the Effect of Point Mutations

Simulation of the Effect of Point Mutations on the Stability of Protein Dimers Using the Bcl-2 Protein Family as an Example
A new method has been developed that enables synthesizing peptides with desired physicochemical properties, for example, with high affinity to one target protein and low affinity to other proteins, and determining the stability of protein complexes with point substitutions of amino acid residues taking into account the three-dimensional structure of the complex by the example of the Bcl2 family, thereby achieving targeted therapeutic selectivity in the treatment of various pathologies
  • Fig. 1. Diagram of formation of a Nap1–Nap1 homodimer
    This study consists of several parts. In the first part,
    the structure and functions of Nap1 protein is
    described. The second part is devoted to the behavior
    of hydrophobic molecules in aqueous environment.
    The third part includes analysis of interaction of two
    proteins using the example of Nap1–Nap1 homodimer formation. In the fourth part, the formation of a hydrophobic cluster is given due to several replacements of amino acids in proteins.
  • Fig. 4. 3D graph of the energy of paired electrostatic interaction
    Fig. 4 shows the map of potential
    energy of electrostatic interaction, where various color
    bars can be observed, the height of which corresponds to a specific energy value, which was calculated between each pair of amino acid residues of two polypeptide chains. The plot shows diagonal peaks (disturbances). The graphical representation allowed us to analyze the effect of point replacements of amino acid residues in polypeptide chains of proteins (Subection 4.1).
  • Fig. 6. Section of polypeptide chains of Nap1 and Nap1
    proteins with indication of key amino acids during replacement
    of T101A
    Figure 6 shows the region of two polypeptide
    chains of Nap1 and Nap1 proteins with indication of
    key amino acids, as well as indication of the change of
    potential energy of electrostatic interaction before and
    after replacement of T101A.
Replacement of Hydrophilic T101A Amino Acid by Hydrophobic Amino Acid Residue

During the interaction of wild-type Nap1–Nap1
proteins, T101 (threonine 101) is characterized by a
sufficiently high negative value of potential energy
with K152 as compared to interactions of other amino
acids; thus, hydrophilic threonine was replaced by
hydrophobic alanine (A) and the potential energy of
electrostatic interaction for such a replacement was
recalculated.

As follows from Table 2, with the replacement of
T101A, there was an increase in the magnitude of
potential energy of interaction. The values of potential
energy in the positive range of values corresponding to
the interaction of hydrophobic amino acids also
appeared, which is considered as "attraction" in aqueous
medium.

Replacement of Hydrophilic T101A Amino Acid by Hydrophobic Amino Acid Residue
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