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使用稳定同位素和质谱法直接测量人类极低密度脂蛋白中载脂蛋白B的合成。

Direct measurement of apolipoprotein B synthesis in human very low density lipoprotein using stable isotopes and mass spectrometry.

作者信息

Cryer D R, Matsushima T, Marsh J B, Yudkoff M, Coates P M, Cortner J A

出版信息

J Lipid Res. 1986 May;27(5):508-16.

PMID:3734634
Abstract

Stable isotope methodology has been adapted to the study of lipoprotein turnover in human subjects. Using endogenous [15N]glycine labeling and gas-liquid chromatographic-mass spectrometric analysis, synthesis of apolipoprotein B in very low density lipoprotein (VLDL) was measured directly in five normal and two hyperlipidemic subjects. An isotopic precursor steady state was achieved during the studies by utilizing a priming dose and constant infusion containing [15N]glycine. Measurement of the plateau in 15N enrichment in the urinary hippurate produced during each study was used to estimate the 15N enrichment of the hepatic glycine precursor pool. The range of values for the fractional synthetic rate of VLDL apoB in the normal subjects obtained by this method was 5.9 to 11.5 day-1, with a mean of 9.2 +/- 2.4 (SD). This value agrees with the results of previous investigations which have utilized other methods. The method was also tested in two hypertriglyceridemic subjects and gave fractional synthetic rates of VLDL apoB that were significantly lower than in normals (1.5 and 2.8 day-1). This stable isotope method allows calculation of the fractional synthetic rate of VLDL apoB by maintaining an isotopic steady state throughout the study. It makes possible repeated studies in the same individual since no risk of exposure to radioisotopes is involved.

摘要

稳定同位素方法已被应用于人体脂蛋白周转的研究。通过内源性[15N]甘氨酸标记和气液色谱 - 质谱分析,在五名正常受试者和两名高脂血症受试者中直接测量了极低密度脂蛋白(VLDL)中载脂蛋白B的合成。在研究过程中,通过使用含有[15N]甘氨酸的起始剂量和持续输注来实现同位素前体稳态。通过测量每次研究期间产生的尿马尿酸盐中15N富集的平稳期,来估计肝脏甘氨酸前体池的15N富集。用这种方法获得的正常受试者中VLDL载脂蛋白B的分数合成率值范围为5.9至11.5天-1,平均值为9.2±2.4(标准差)。该值与先前使用其他方法的研究结果一致。该方法也在两名高甘油三酯血症受试者中进行了测试,得到的VLDL载脂蛋白B的分数合成率明显低于正常受试者(1.5和2.8天-1)。这种稳定同位素方法通过在整个研究过程中保持同位素稳态,从而能够计算VLDL载脂蛋白B的分数合成率。由于不涉及接触放射性同位素的风险,因此可以在同一个体中进行重复研究。

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