首页> 外文期刊>Metabolism: Clinical and Experimental >Postprandial changes in the distribution of apolipoprotein AIV between apolipoprotein b- and non apolipoprotein b-containing lipoproteins in obese women.
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Postprandial changes in the distribution of apolipoprotein AIV between apolipoprotein b- and non apolipoprotein b-containing lipoproteins in obese women.

机译:肥胖妇女餐后餐后载脂蛋白b和非载脂蛋白b脂蛋白之间载脂蛋白AIV分布的变化。

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摘要

Plasma apolipoprotein AIV (apo AIV) level has been shown to be a good marker of triglyceride changes after a high-fat diet. However, the distribution of apo AIV between apo B- and non-apo B-containing lipoproteins (Lp) during the postprandial state has not been described as well as the influence of obesity on this distribution. Our aim was to study the influence of parameters related to obesity and insulin resistance on the postprandial changes in apo AIV-containing Lp after a high-fat meal in obese women. Twenty-three overweight or obese women (body mass index [BMI] ranging from 29.1 and 64.0 kg.1 m(-2)), for whom blood samples were taken after fasting overnight, participated in the study. Thirteen of these obese women were given a fatty meal and, in this case, blood samples were taken at fast and 30 minutes, 1, 2, 4, and 6 hours after ingestion of the fat meal. Apo AIV-containing particle families, Lp B:AIVf (family [f] of particles containing at least apo B and apo AIV) and Lp AIV non-Bf (family [f]of particles containing apo AIV, but free of apo B) were quantified by sandwich enzyme-linked immunosorbent assay (ELISA). When fasting, Lp B:AIVf and Lp AIV non-Bf did not correlate with any of the parameters related to obesity and insulin resistance, if one excepts a positive correlation between HDL-cholesterol (HDL-C) and Lp AIV non-Bf. Postprandial lipemia was associated with a trend towards an increase in the plasma levels of apo AIV-containing Lp 6 hours after fat ingestion. The postprandial peak of Lp B:AIVf and Lp AIV non-Bf occurred 2 hours after the triglyceride peak. The distribution between apo B- and non-apo B-containing Lp did not change after ingestion of the fat meal, if one excepts a tendancy towards a lower ratio of bound and nonbound forms at 8 hours. Fasting plasma Lp B:AIVf concentration correlated with the area under the curve (AUC) of plasma triglycerides (beta = 0.11, P <.02). In a multivariate analysis, BMI (beta = 51.85, P <.001), fasting triglycerides (beta = 431.08, P <.01), and low-density lipoprotein-cholesterol (LDL-C) (beta = 2638.57, P <.005) were independent and positive determinants of the AUC of Lp AIV non-Bf, while waist circumference (beta = -23.94, P <.001), cholesterol (beta = -1655.02, P <.01), and systolic blood pressure (beta = -6.34, P <.05) were negative and independent determinants of this AUC. Fasting Lp B:AIVf may represent a good marker of the postprandial triglyceride increase in obese women. Changes in apo AIV concentrations in apo B- and non-apo B-containing Lp after a fat meal depend mainly on the degree of obesity rather than on insulin resistance. This effect is more obvious for Lp AIV non-Bf than for Lp B:AIVf.
机译:高脂饮食后血浆载脂蛋白AIV(apo AIV)水平已显示是甘油三酸酯变化的良好标志。然而,尚未描述餐后状态期间载脂蛋白B和不载脂蛋白B的脂蛋白(Lp)之间载脂蛋白AIV的分布以及肥胖对这种分布的影响。我们的目的是研究与肥胖和胰岛素抵抗相关的参数对肥胖妇女高脂餐后含apo AIV的Lp餐后变化的影响。二十三名超重或肥胖的妇女(体重指数[BMI]在29.1和64.0 kg.1 m(-2)之间),他们在禁食过夜后抽取了血样,参加了这项研究。这些肥胖妇女中有13名接受了脂肪餐,在这种情况下,在摄取脂肪餐后的第30分钟,1、2、4和6小时快速采集了血样。包含Apo AIV的粒子家族,Lp B:AIVf(至少包含apo B和apo AIV的粒子家族[f])和Lp AIV非Bf(包含apo AIV但不含apo B的粒子家族[f])通过夹心酶联免疫吸附测定(ELISA)定量。禁食时,如果HDP胆固醇(HDL-C)与Lp AIV非Bf之间呈正相关,则Lp B:AIVf和Lp AIV非Bf与肥胖和胰岛素抵抗相关的任何参数均不相关。餐后脂肪血症与脂肪摄入后6小时血浆含apo AIV的Lp血浆水平升高的趋势有关。 Lp B:AIVf和Lp AIV non-Bf的餐后峰值出现在甘油三酸酯峰值后2小时。摄入脂肪粉后,载脂蛋白B和不含载脂蛋白B的Lp之间的分布没有变化,除非有人倾向于在8小时时趋向于结合和非结合形式的比例降低。空腹血浆Lp B:AIVf浓度与血浆甘油三酸酯的曲线下面积(AUC)相关(β= 0.11,P <.02)。在多变量分析中,BMI(beta = 51.85,P <.001),空腹甘油三酸酯(beta = 431.08,P <.01)和低密度脂蛋白胆固醇(LDL-C)(beta = 2638.57,P <。 005)是Lp AIV非Bf的AUC的独立和阳性决定因素,而腰围(β= -23.94,P <.001),胆固醇(β= -1655.02,P <.01)和收缩压( β= -6.34,P <.05)是该AUC的阴性和独立决定因素。空腹Lp B:AIVf可能代表肥胖女性餐后甘油三酯增加的良好标志。脂肪餐后含apo B和不含apo B的Lp中apo AIV浓度的变化主要取决于肥胖程度,而不是胰岛素抵抗。对于Lp AIV non-Bf,此作用比Lp B:AIVf更明显。

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