Urinary prostaglandin E2 and vasopressin excretion in essential fatty acid-deficient rats: Effect of linolenic acid supplementation

Abstract

Three groups of weanling male rats were fed on a fat-free diet for 13 weeks. One group received only the fat-free diet (FF rats), the other 2 groups received the fat-free diet and a daily supplement of 2 energy% ethyl linoleate ([n−6] rats), or 2 energy% ethyl linolenate ([n−3] rats). Urinary excretion of prostaglandin E₂ (PGE₂), immunoreactive arginine vasopressin (iA VP), and kallikrein were determined. PGE₂ was quantitated with a radioimmunoassay having 4.9% cross-reactivity with prostaglandin E₃ (PGE₃). After 4 weeks on the diet, water consumption and urinary iAVP excretion increased significantly in the FF rats and the (n−3) rats compared with the (n−6) rats. Urinary PGE₂ excretion was the same for all 3 groups during the first 10 weeks; thereafter it decreased in FF rats and (n−3) rats compared with the (n−6) rats. There was no difference in urinary PGE₂ excretion between the FF rats and the (n−3) rats, even though large differences were found in the percentage of arachidonic acid (20∶4[n−6]), icosapentaenoic acid (20∶5[n−3]), and icosatrienoic acid (20∶3[n−9]) of total kidney fatty acids as well as of kidney phosphatidylinositol fatty acids. Fractionation of urine extracts on high performance liquid chromatography with radioimmunoassay detection indicated that (n−3) rats excreted very little PGE₃, if any. Urine output followed the same pattern, as did urinary PGE₂ excretion. Urinary kallikrein was estimated at week 12 only. It was found to be significantly lower in FF rats and (n−3) rats. Increased water consumption and increased urinary iAVP excretion seem to be early symptoms (after 4 weeks) of EFA deficiency, whereas decreased urine output and decreased urinary PGE₂ excretion occur much later (after 10 weeks). Two energy% linolenate supplementation to a fat-free diet did not change the appearance of any of the measured EFA-deficiency symptoms except for a slightly improved growth rate. There was no evidence of a significant urinary PGE₃ excretion in spite of an extreme enrichment of kidney lipids with 20∶5(n−3). It is suggested that urinary PGE₂ is derived from precursors delivered from an arachidonic acid pool, which is rather resistant to restriction in dietary linoleate.