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泌乳奶牛体内肉豆蔻酸、棕榈酸和硬脂酸Δ9-去饱和作用的活体测量方法。

Methodology for the in vivo measurement of the delta9-desaturation of myristic, palmitic, and stearic acids in lactating dairy cattle.

作者信息

Mosley Erin E, McGuire Mark A

机构信息

Department of Animal and Veterinary Science, University of Idaho, PO Box 442330, Moscow, ID 83844-2330, USA.

出版信息

Lipids. 2007 Oct;42(10):939-45. doi: 10.1007/s11745-007-3085-x. Epub 2007 Jul 6.

DOI:10.1007/s11745-007-3085-x
PMID:17619092
Abstract

There is limited methodology available to quantitatively assess the activity of the Delta9-desaturase enzyme in vivo without chemically inhibiting the enzyme or using radioactively labeled substrates. The objective of these experiments was to develop methodology to determine the incorporation and desaturation of 13C-labeled fatty acids into milk lipids. In a preliminary experiment, 3.7 g [1-13C]myristic acid ([1-13C]14:0), 19.5 g [1-13C]palmitic acid ([1-13C]16:0), 20.0 g [1-13C]stearic acid ([1-13C]18:0) were combined and infused into the duodenum of a cow over 24 h. In a following experiment, 5.0 g [1-13C]14:0, 40.0 g [1-13C]16:0, and 50.0 g [1-13C]18:0 were infused into the abomasums of separate cows as a bolus over 20 min or continuously over 24 h. Milk fat was extracted using chloroform:methanol. Fatty acids were methylated, and fatty acid methyl esters (FAME) were converted to dimethyl disulfide derivatives (DMDS). The FAME and DMDS were analyzed by gas chromatography mass spectrometry. In the preliminary experiment, 13C enrichment in 14:0 but not 16:0 or 18:0 was observed. When dosage amounts were increased in the following experiment, peak enrichments from the bolus infusion were observed at 8 h. Enrichments for continuous infusion peaked at 16 h for 14:0 and 18:0, and at 24 h for 16:0. The Delta9-desaturase products of these fatty acids were estimated to be 90% of cis-9 14:1, 50% of cis-9 16:1, and 59% of cis-9 18:1. This study demonstrates that 13C-labeled fatty acids may be utilized in vivo to measure the activity of the Delta9-desaturase enzyme.

摘要

在不使用化学方法抑制该酶或不使用放射性标记底物的情况下,用于在体内定量评估Δ9-去饱和酶活性的方法有限。这些实验的目的是开发一种方法,以确定13C标记的脂肪酸掺入乳脂并进行去饱和的情况。在一个初步实验中,将3.7克[1-13C]肉豆蔻酸([1-13C]14:0)、19.5克[1-13C]棕榈酸([1-13C]16:0)、20.0克[1-13C]硬脂酸([1-13C]18:0)混合,并在24小时内注入一头奶牛的十二指肠。在接下来的实验中,将5.0克[1-13C]14:0、40.0克[1-13C]16:0和50.0克[1-13C]18:0作为大剂量在20分钟内或在24小时内连续注入不同奶牛的皱胃。使用氯仿:甲醇提取乳脂肪。脂肪酸进行甲基化,脂肪酸甲酯(FAME)转化为二甲基二硫衍生物(DMDS)。通过气相色谱-质谱联用仪分析FAME和DMDS。在初步实验中,观察到14:0中有13C富集,但16:0和18:0中没有。在接下来的实验中增加剂量时,大剂量注入后8小时观察到峰值富集。连续注入时,14:0和18:0在16小时达到富集峰值,16:0在24小时达到富集峰值。这些脂肪酸的Δ9-去饱和酶产物估计分别为顺式-9 14:1的90%、顺式-9 16:1的50%和顺式-9 18:1的59%。这项研究表明,13C标记的脂肪酸可用于体内测量Δ9-去饱和酶的活性。

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