Bailhache E, Briand F, Nguyen P, Krempf M, Magot T, Ouguerram K
Centre de Recherche en Nutrition Humaine, INSERM U539, CHU Nantes, France.
Eur J Clin Invest. 2004 Aug;34(8):527-34. doi: 10.1111/j.1365-2362.2004.01387.x.
It has been shown that dogs exhibit no cholesterol ester transfer protein (CETP) activity in vitro, in contrast to humans. The aim of our study was to determine modalities of in vivo plasma cholesterol ester turnover in this species, using a kinetic approach with stable isotopes.
Kinetics of very low-density lipoprotein (VLDL) and low-density lipoprotein (LDL) were studied in seven adult male Beagle dogs using a dual isotope approach through endogenous labelling of both their cholesterol moiety and their protein moiety. A primed constant infusion of both [1,2(13)C]acetate and [5,5,5-2H3]leucine enabled us to obtain measurable deuterium enrichments by gas chromatography-mass spectrometry for plasma leucine and apoB100, as well as measurable 13C enrichment by gas chromatography-combustion-isotopic ratio mass spectrometry for unesterified cholesterol and cholesterol ester in the VLDL and LDL. Two identical multicompartmental models (SAAM II) were used together for the analysis of tracer kinetics' data of proteins and cholesterol.
Characterization of the apoB100-containing lipoprotein cholesterol ester model allowed determination of kinetic parameters of VLDL and LDL cholesterol ester metabolism. We succeeded in modelling VLDL and LDL cholesterol ester metabolism and apoB100 metabolism simultaneously. Fractional catabolic rate (FCR) of apoB100 and CE had the same values. Introducing cholesterol ester transfer between lipoproteins in the model did not significantly improve the fit. Total VLDL FCR was 2.97 +/- 01.47 h(-1). Approximately one-quarter corresponded to the direct removal of VLDL (0.81 +/- 00.34 h(-1)) and the remaining three-quarters corresponded to the fraction of VLDL converted to LDL, which represented a conversion of VLDL into LDL of 2.16 +/- 01.16 h(-1). Low-density lipoproteins were produced exclusively from VLDL conversion and were then removed (0.031 +/- 0.004 h(-1)) from plasma.
These kinetic data showed that VLDL cholesterol ester and LDL cholesterol ester metabolism followed VLDL and LDL apoB100 metabolism, and that consequently there is no in vivo transfer of cholesterol ester in dogs.
与人类不同,已有研究表明犬类在体外不表现出胆固醇酯转运蛋白(CETP)活性。我们研究的目的是采用稳定同位素动力学方法,确定该物种体内血浆胆固醇酯周转的方式。
使用双同位素方法,通过对极低密度脂蛋白(VLDL)和低密度脂蛋白(LDL)的胆固醇部分和蛋白质部分进行内源性标记,研究了7只成年雄性比格犬的VLDL和LDL动力学。同时给予[1,2(13)C]乙酸盐和[5,5,5-2H3]亮氨酸的预充恒定输注,使我们能够通过气相色谱-质谱法测定血浆亮氨酸和载脂蛋白B100的可测量氘富集,以及通过气相色谱-燃烧-同位素比率质谱法测定VLDL和LDL中游离胆固醇和胆固醇酯的可测量13C富集。使用两个相同的多室模型(SAAM II)共同分析蛋白质和胆固醇的示踪动力学数据。
含载脂蛋白B100的脂蛋白胆固醇酯模型的表征使得能够确定VLDL和LDL胆固醇酯代谢的动力学参数。我们成功地同时对VLDL和LDL胆固醇酯代谢以及载脂蛋白B100代谢进行了建模。载脂蛋白B100和胆固醇酯的分解代谢率(FCR)值相同。在模型中引入脂蛋白之间的胆固醇酯转移并没有显著改善拟合效果。总VLDL FCR为2.97±0.147 h(-1)。大约四分之一对应于VLDL的直接清除(0.81±0.034 h(-1)),其余四分之三对应于转化为LDL的VLDL部分,这代表VLDL向LDL的转化率为2.16±0.116 h(-1)。低密度脂蛋白仅由VLDL转化产生,然后从血浆中清除(0.031±0.004 h(-1))。
这些动力学数据表明,VLDL胆固醇酯和LDL胆固醇酯代谢遵循VLDL和LDL载脂蛋白B100代谢,因此犬体内不存在胆固醇酯的体内转移。
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