Women aged less than 40 have higher docosahexaenoic acid (22:6n-3) status( Reference Burdge and Wottoon 1 ) and convert more 18:3n-3 to longer chain n-3 polyunsaturated fatty acids (PUFA) than men( Reference Burdge, Jones and Wottoon 2 ). Female rats also have higher liver and plasma phospholipid 22:6n-3 status than males( Reference Childs, Romeu-Nadal and Burdge 3 ). Greater PUFA biosynthesis in women involves increased conversion of 22:5n-3 to 22:6n-3( Reference Pawlosky, Hibbeln and Lin 4 ), and female sex hormones have been shown to increase plasma 22:6n-3 concentration and to up-regulate 22:6n-3, although the precise mechanism remains unclear( Reference Giltay, Gooren and Toorians 5 ). It is not known when in the life course the sexual divergence in 22:6n-3 status and PUFA biosynthesis is induced. We hypothesised that puberty is the key period in which capacity for 22:6n-3 synthesis and status increases in females. To test this, we compared the liver fatty acid composition of juvenile and adult male and female rats.
Pregnant and lactating Wistar rats were fed a semi-purified diet (AIN93G) throughout gestation. Offspring were either weaned on postnatal d28 onto AIN93M or killed on postnatal d70 (n 7 males or females per age group, one male or female per litter). Livers were collected, snap frozen and the fatty acid composition of liver phosphatidylcholine (PC) was measured by gas chromatography( Reference Burdge 6 ).
There was a significant interaction effect of age*sex on the proportion of 18:3n-3 (P=0.027) and 20:5n-3 (P=0.009) in liver PC such that the proportions of these fatty acids were higher in d28 females and in d70 males and females compared to d28 males (Figs. 1 and 2). There was a significant effect of age (P<0.001), but not sex, on proportion of 22:5n-3 in liver PC such that it was lower d70 liver compared to d28 (Fig. 3). There was a significant age*sex interaction (P=0.001) on proportion of 22:6n-3 in liver PC. The proportion of 22:6n-3 was significantly greater at d28 compared to d70 irrespective of sex. The proportion of 22:6n-3 in liver PC was higher in adult females than males, but did not differ between sexes at d28 (Fig. 4).
Fig. 1. Liver PC 18:3n-3.
Fig. 2. Liver PC 20:5n-3.
Fig. 3. Liver PC 22:5n-3.
Fig. 4. Liver PC 22:6n-3.
Values are mean (SD). Data were analysed by two-way ANOVA with sex and age as fixed factors, with Bonferroni's post hoc test. Means with different letters differed significantly (P<0.05).
These findings show that both age and sex affect the proportions of n-3 PUFA in liver in a manner contingent on the fatty acid species. As in human plasma PC( Reference Burdge and Calder 7 ), the proportion of 20:5n-3 in rat liver PC appears to be related to 18:3n-3 status. Synthesis of 22:5n-3 and 22:6n-3 appeared to be independent of 20:5n-3 status and to be down-regulated in adults compared to juveniles. The sex difference in the proportion of 22:6n-3, but not 22:5n-3, in adults is consistent with greater conversion of 22:5n-6 to 22:6n-3 in women than men( Reference Burdge and Wottoon 1 – Reference Pawlosky, Hibbeln and Lin4 )and with the suggestion that these metabolic reactions are regulated independently of the conversion of 18:3n-3 to 20:5n-3( Reference Sprecher and Baykousheva 8 ). Our findings support the suggestion that puberty represents an important influence on PUFA metabolism which acts through several regulatory loci.
