Fasting hepatic de novo lipogenesis is not reliably assessed using circulating fatty acid markers

被引:18
|
作者
Rosqvist, Fredrik [1 ,2 ]
McNeil, Catriona A. [1 ]
Pramfalk, Camilla [1 ,3 ]
Parry, Sion A. [1 ]
Low, Wee Suan [1 ]
Cornfield, Thomas [1 ]
Fielding, Barbara A. [4 ]
Hodson, Leanne [1 ,5 ]
机构
[1] Univ Oxford, Churchill Hosp, Oxford Ctr Diabet Endocrinol & Metab, Oxford, England
[2] Uppsala Univ, Dept Publ Hlth & Caring Sci, Clin Nutr & Metab, Uppsala, Sweden
[3] Karolinska Univ Hosp Huddinge, Karolinska Inst, Div Clin Chem, Dept Lab Med, Stockholm, Sweden
[4] Univ Surrey, Fac Hlth & Med Sci, Guildford, Surrey, England
[5] Churchill Hosp, Oxford NIHR Biomed Res Ctr, Oxford, England
基金
英国生物技术与生命科学研究理事会;
关键词
de novo lipogenesis; fatty acids; metabolism; human; triglycerides; lipogenic index; SCD; palmitoleic acid; ADIPOSE-TISSUE; VLDL-TRIGLYCERIDE; HUMAN PLASMA; LIVER; BLOOD; PATHWAY; RISK; LIPOPROTEINS; CHOLESTEROL; CONTRIBUTES;
D O I
10.1093/ajcn/nqy304
中图分类号
R15 [营养卫生、食品卫生]; TS201 [基础科学];
学科分类号
100403 ;
摘要
Background: Observational studies often infer hepatic de novo lipogenesis (DNL) by measuring circulating fatty acid (FA) markers; however, it remains to be elucidated whether these markers accurately reflect hepatic DNL. Objectives: We investigated associations between fasting hepatic DNL and proposed FA markers of DNL in subjects consuming their habitual diet. Methods: Fasting hepatic DNL was assessed using (H2O)-H-2(deuterated water) in 149 nondiabetic men and women and measuring the synthesis of very low-density lipoprotein triglyceride (VLDL-TG) palmitate. FA markers of blood lipid fractions were determined by gas chromatography. Results: Neither the lipogenic index (16: 0/18: 2n-6) nor the SCD index (16: 1n-7/16: 0) in VLDL-TG was associated with isotopically assessed DNL (r = 0.13, P = 0.1 and r = -0.08, P = 0.35, respectively). The relative abundances (mol%) of 14: 0, 16: 0, and 18: 0 in VLDL-TG were weakly (r <= 0.35) associated with DNL, whereas the abundances of 16: 1n-7, 18: 1n-7, and 18: 1n-9 were not associated. When the cohort was split by median DNL, only the abundances of 14: 0 and 18: 0 in VLDL-TG could discriminate between subjects having high (11.5%) and low(3.8%) fasting hepatic DNL. Based on a subgroup, FA markers in total plasma TG, plasma cholesteryl esters, plasma phospholipids, and red blood cell phospholipids were generally not associated with DNL. Conclusions: The usefulness of circulating FAs as markers of hepatic DNL in healthy individuals consuming their habitual diet is limited due to their inability to discriminate clearly between individuals with low and high fasting hepatic DNL.
引用
收藏
页码:260 / 268
页数:9
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