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首页> 美国卫生研究院文献>other >Regulation of Tissue LC-PUFA Contents Δ6 Fatty Acyl Desaturase (FADS2) Gene Expression and the Methylation of the Putative FADS2 Gene Promoter by Different Dietary Fatty Acid Profiles in Japanese Seabass (Lateolabrax japonicus)
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Regulation of Tissue LC-PUFA Contents Δ6 Fatty Acyl Desaturase (FADS2) Gene Expression and the Methylation of the Putative FADS2 Gene Promoter by Different Dietary Fatty Acid Profiles in Japanese Seabass (Lateolabrax japonicus)

机译:日本鲈鱼(Lateolabrax japonicus)不同饮食脂肪酸谱对组织LC-PUFA含量Δ6脂肪酰基去饱和酶(FADS2)基因表达和推定FADS2基因启动子甲基化的调节

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The present study was conducted to evaluate the influences of different dietary fatty acid profiles on the tissue content and biosynthesis of LC-PUFA in a euryhaline species Japanese seabass reared in seawater. Six diets were prepared, each with a characteristic fatty acid: Diet PA: Palmitic acid (C16:0); Diet SA: Stearic acid (C18:0); Diet OA: Oleic acid (C18:1n-9); Diet LNA: α-linolenic acid (C18:3n-3); Diet N-3 LC-PUFA: n-3 LC-PUFA (DHA+EPA); Diet FO: the fish oil control. A 10-week feeding trial was conducted using juvenile fish (29.53±0.86 g). The results showed that Japanese seabass had limited capacity to synthesize LC-PUFA and fish fed PA, SA, OA and LNA showed significantly lower tissue n-3 LC-PUFA contents compared to fish fed N-3 LC-PUFA and FO. The putative gene promoter and full-length cDNA of FADS2 was cloned and characterized. The protein sequence was confirmed to be homologous to FADS2s of marine teleosts and possessed all the characteristic features of microsomal fatty acid desaturases. The FADS2 transcript levels in liver of fish fed N-3 LC-PUFA and FO were significantly lower than those in fish fed other diets except LNA while Diet PA significantly up-regulated the FADS2 gene expression compared to Diet LNA, N-3 LC-PUFA and FO. Inversely, fish fed N-3 LC-PUFA and FO showed significantly higher promoter methylation rates of FADS2 gene compared to fish fed the LC-PUFA deficient diets. These results suggested that Japanese seabass had low LC-PUFA synthesis capacity and LC-PUFA deficient diets caused significantly reduced tissue n-3 LC-PUFA contents. The liver gene expression of FADS2 was up-regulated in groups enriched in C16:0, C18:0 and C18:1n-9 respectively but not in the group enriched in C18:3n-3 compared to groups with high n-3 LC-PUFA contents. The FADS2 gene expression regulated by dietary fatty acids was significantly negatively correlated with the methylation rate of putative FADS2 gene promoter.
机译:本研究旨在评估不同饮食脂肪酸谱对海水中养成的日本淡水鲈鱼组织中LC-PUFA的含量和生物合成的影响。制备了六种饮食,每种饮食均具有特征性脂肪酸:饮食PA:棕榈酸(C16:0); Diet SA:硬脂酸(C18:0);饮食OA:油酸(C18:1n-9);饮食LNA:α-亚麻酸(C18:3n-3);饮食N-3 LC-PUFA:n-3 LC-PUFA(DHA + EPA);饮食FO:鱼油的控制。使用幼鱼(29.53±0.86 g)进行了为期10周的饲养试验。结果表明,日本鲈鱼合成LC-PUFA的能力有限,与饲喂N-3 LC-PUFA和FO的鱼相比,饲喂PA,SA,OA和LNA的鱼的n-3 LC-PUFA组织含量低得多。克隆并鉴定了FADS2的推定基因启动子和全长cDNA。该蛋白序列被证实与海洋硬骨鱼的FADS2同源,并具有微粒体脂肪酸去饱和酶的所有特征。饲喂N-3 LC-PUFA和FO的鱼肝脏中的FADS2转录水平显着低于饲喂LNA以外的其他饮食的鱼,而Diet PA与Diet LNA,N-3 LC-相比显着上调了FADS2基因的表达。 PUFA和FO。相反,饲喂N-3 LC-PUFA和FO的鱼与饲喂LC-PUFA缺乏饮食的鱼相比,FADS2基因的启动子甲基化率明显更高。这些结果表明,日本鲈鱼的LC-PUFA合成能力低,且LC-PUFA缺乏饮食会导致组织中n-3 LC-PUFA含量显着降低。与具有高n-3 LC-值的组相比,分别富集C16:0,C18:0和C18:1n-9的组中FADS2的肝基因表达上调,而富集C18:3n-3的组则没有上调。 PUFA内容。膳食脂肪酸调节的FADS2基因表达与推定的FADS2基因启动子的甲基化率显着负相关。

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