Effects of urea and trimethylamine N-oxide on fluidity of liposomes and membranes of an elasmobranch

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Am J Physiol Regul Integr Comp Physiol 276: R397-R406, 1999;
0363-6119/99 $5.00

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Vol. 276, Issue 2, R397-R406, February 1999

Effects of urea and trimethylamine N-oxide on fluidity of liposomes and membranes of an elasmobranch

Kimby N. Barton¹, Mary M. Buhr², and James S. Ballantyne¹

¹ Departments of Zoology and ² Animal and Poultry Science, University of Guelph, Guelph, Ontario, Canada N1G 2W1

The effects on membrane fluidity of two solutes of biological importance in elasmobranch fishes, urea and trimethylamine oxide(TMAO), were determined using elasmobranch red blood cell plasmamembranes and artificial liposomes. Fluorescence polarizationsof three probes with differing sites of insertion (1,6-diphenylhexatriene,cis-parinaric acid, and trans-parinaric acid) were used to studythe effects of physiological levels of urea (400 mM) and TMAO(200 mM) separately and together in a 2:1 urea:TMAO ratio (400mM:200 mM). In the elasmobranch erythrocyte membrane, there wasa trend toward an increase in the order of the gel-phase domainswhen treated with urea, although this was not statistically significant.This effect was counteracted by the presence of TMAO. To determineif the organic solutes were acting directly on the membrane lipidsor on the integral proteins, phase-transition profiles of protein-freedipalmitoyl phosphatidylcholine liposomes were determined. Theseprofiles showed that urea again increased the order of the gel-phasedomains of the bilayer; however, this effect was not counteractedby the presence of TMAO. We suggest that the increased order inthe gel-phase domains may be an indirect effect of a decreasein the order of the fluid-phase domains. This increase in fluiditymay be due either to a disruptive effect of urea on the hydrophobiccore of the membrane or to indirect effects mediated by changesin the integral membrane proteins. This study is the first todemonstrate that urea and TMAO may act as counteracting solutesin the elasmobranch erythrocyte membrane and that the counteractionappears to be at the level of the integral proteins rather thanthe membranelipids.

organic solutes; membrane adaptation; lipid; fluorescence polarization

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