肝脏极低密度脂蛋白三酰甘油的起源:细胞磷脂的作用。
Origin of hepatic very-low-density lipoprotein triacylglycerol: the contribution of cellular phospholipid.
作者信息
Wiggins D, Gibbons G F
机构信息
Nuffield Department of Clinical Medicine, University of Oxford, Radclifle Infirmary.
出版信息
Biochem J. 1996 Dec 1;320 ( Pt 2)(Pt 2):673-9. doi: 10.1042/bj3200673.
When rat hepatocytes were cultured for 24 h in the absence of exogenous fatty acid, the amount of very-low-density lipoprotein (VLDL) triacylglycerol (TAG) secreted (114 +/- 14 micrograms/mg of cell protein) could not be accounted for by the mass of TAG lost from the cells (29 +/- 6.1 micrograms/mg of cell protein) during this period (n = 12). Of the balance (85 +/- 14 micrograms/mg; 94 +/- 15 nmol/mg), a maximum of only 37 nmol/mg of cell protein of TAG could be accounted for by fatty acids synthesized de novo. When labelled exogenous oleate (initial concentration, 0.75 nM) was present in the culture medium, the net gain in cellular plus VLDL TAG (253 +/- 38 micrograms/mg of cell protein per 24 h) was greater than that contributed by the exogenous fatty acid (155 +/- 18.2 micrograms/mg of cell protein, n = 5). Again, the balance (98.8 +/- 18.2 micrograms/mg of cell protein per 24 h) was too great to be accounted for by fatty acid synthesis de novo. In experiments in which cellular glycerolipids were prelabelled with [9, 10(n)-3H]oleic acid, following removal of the labelled fatty acid, there was a net increase in labelled cellular plus VLDL TAG over the next 24 h. That cellular phospholipids are the source of a substantial part of the excess TAG synthesized is supported by the following evidence. (1) The loss of prelabelled cellular phospholipid during culture was greater than could be accounted for by secretion into the medium. (2) During culture of cells prelabelled with 1,2-di-[l-14C]palmitoyl phosphatidylcholine, a substantial amount of label was secreted as VLDL TAG. (3) In pulse-chase experiments, the kinetics of labelled phospholipid turnover were consistent with conversion into a non-phospholipid pool. The enzymology involved in the transfer of phospholipid fatty acids into TAG is probably complex, but the present results suggest that this pathway may represent an important route by which extracellular fatty acids are channelled into VLDL TAG.
当大鼠肝细胞在无外源脂肪酸的情况下培养24小时时,分泌的极低密度脂蛋白(VLDL)三酰甘油(TAG)量(114±14微克/毫克细胞蛋白)无法用此期间细胞中损失的TAG量(29±6.1微克/毫克细胞蛋白)来解释(n = 12)。在剩余部分(85±14微克/毫克;94±15纳摩尔/毫克)中,从头合成的脂肪酸最多只能解释37纳摩尔/毫克细胞蛋白的TAG。当培养基中存在标记的外源油酸(初始浓度为0.75纳摩尔)时,细胞加VLDL TAG的净增加量(每24小时253±38微克/毫克细胞蛋白)大于外源脂肪酸的贡献量(155±18.2微克/毫克细胞蛋白,n = 5)。同样,剩余部分(每24小时98.8±18.2微克/毫克细胞蛋白)太大,无法用从头合成脂肪酸来解释。在用[9,10(n)-3H]油酸对细胞甘油脂质进行预标记的实验中,去除标记脂肪酸后,在接下来的24小时内,标记的细胞加VLDL TAG出现净增加。以下证据支持细胞磷脂是合成的过量TAG的主要来源这一观点。(1)培养过程中预标记的细胞磷脂损失量大于分泌到培养基中的量。(2)在用1,2-二-[l-14C]棕榈酰磷脂酰胆碱预标记的细胞培养过程中,大量标记物以VLDL TAG的形式分泌。(3)在脉冲追踪实验中,标记磷脂周转的动力学与转化为非磷脂池一致。磷脂脂肪酸向TAG转移所涉及的酶学可能很复杂,但目前的结果表明,这条途径可能是细胞外脂肪酸进入VLDL TAG的重要途径。
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