The bacteriolytic activity of interleukin-2 and chicken egg lysozyme in the
presence of various substances has been studied. Glycine and lysine do not
affect the activity of interleukin-2 but increase that of lysozyme, showing a
bell-shape concentration dependence peaking at 1.5 mM glycine and 18 mM lysine.
Arginine and glutamate activate both interleukin-2 and lysozyme with a
concentration dependence of the saturation type. Aromatic amino acids have
almost no effect on the activity of both interleukin-2 and lysozyme. Aromatic
amines, tryptamine, and tyramine activate interleukin-2 but inhibit lysozyme.
Peptide antibiotics affect interleukin and lysozyme similarly and exhibit
maximum activity in the micromolar range of antibiotics. Taurine has no effect
on the activity of interleukin-2 and lysozyme. Mildronate showed no influence
on lysozyme, but it activated interleukin-2 with the activity maximum at 3 mM.
EDTA activates both interleukin-2 and lysozyme at concentrations above 0.15 mM.
In order to accelerate Sodium dodecyl sulfate–polyacrylamide gel electrophoresis (SDS–PAGE), here we propose an optimized version of the technique enabled by experimental tuning reinforced by theoretical description. In the resulting system, the gel buffer was diluted twofold and supplemented with glycine at a low concentration, whereas a higher voltage was applied. This approach reduced runtime from 90 to 18 min. It is important to emphasize that, despite the high voltage applied to the gel, the resolution of the bands did not decrease compared to the original Laemmli method. The proposed acceleration approach can be used in other variants of SDS–PAGE.
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