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Why is glycine not a part of the osmoticum in the urea-rich cells?

Protein and peptide letters (2012-06-08)
Sheeza Khan, Zehra Bano, Laishram R Singh, Md Imtaiyaz Hassan, Asimul Islam, Faizan Ahmad
ABSTRACT

Kidney cells of animals including human and marine invertebrates contain high amount of the protein denaturant, urea. Methylamine osmolytes are generally believed to offset the harmful effects of urea on proteins in vitro and in vivo. In this study we have investigated the possibility of glycine to counteract the effects of urea on three proteins by measuring thermodynamic stability, ΔGD° and functional activity parameters (K(m) and k(cat)). We discovered that glycine does not counteract the effects of urea in terms of both protein stability and functional activity. We also observed that the glycine alone is compatible with enzymes function and increases protein stability in terms of T(m) (midpoint of thermal denaturation) to a great extent. Our study indicates that a most probable reason for the absence of a stabilizing osmolyte, glycine in the urea-rich cells is due to the fact that this osmolyte is non-protective to macromolecules against the hostile effects of urea, and hence is not chosen by evolutionary selection pressure.

MATERIALS
Product Number
Brand
Product Description

Sigma-Aldrich
Methylamine-13C hydrochloride, 99 atom % 13C
Sigma-Aldrich
Methylamine solution, 33 wt. % in absolute ethanol ((denatured with 1% toluene))
Sigma-Aldrich
Methylamine solution, 2.0 M in methanol
Sigma-Aldrich
Methylamine solution, 40 wt. % in H2O
Sigma-Aldrich
Methylamine solution, 2.0 M in THF
Sigma-Aldrich
Methylamine-15N hydrochloride, 98 atom % 15N
Sigma-Aldrich
Methylamine hydrochloride, ≥98%