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豚鼠低密度脂蛋白:结构与代谢的异质性

Guinea pig low density lipoproteins: structural and metabolic heterogeneity.

作者信息

Luc G, Chapman M J

机构信息

Groupe de Recherches INSERM sur les Lipoprotéines, Pavillon Benjamin Delessert, Hôpital de la Pitiè, Paris, France.

出版信息

J Lipid Res. 1988 Oct;29(10):1251-63.

PMID:2466928
Abstract

The structural and metabolic heterogeneity of low density lipoproteins (LDL, d 1.024-1.100 g/ml) has been investigated in the guinea pig. Two LDL subfractions, of d 1.024-1.050 and 1.050-1.100 g/ml, respectively, were isolated by sequential ultracentrifugation; while both were enriched in cholesteryl ester and apoB-100, the former was heterogeneous displaying three particle size species of diameters 26.9, 25.6, and 24.7 nm, whereas the denser subfraction was relatively homogeneous containing a single, smaller species (diam. 23.6 nm). The fractional catabolic rates (FCR) of the two LDL subfractions were alike (approximately 0.090 pools/hr) in the guinea pig in vivo. After modification of each subfraction by reductive methylation, the FCRs were reduced similarly and indicated that 70-80% of degradation occurred via the cellular LDL receptor pathway. However, the intravascular metabolism of these LDL subfractions, determined from the radioactive content of density gradient fractions as a function of time after injection of radiolabeled native or chemically modified LDL, tended to be distinct. Thus, while radiolabeled apoB-100 in the lighter subfraction maintained the initial density profile up to 48 hr, the radioactive profile of its methylated counterpart changed, the proportion of radioactivity in the lighter gradient fractions (d 1.027-1.032 g/ml) increasing while that in the denser (d 1.037-1.042 g/ml) fractions diminished. A more marked transformation occurred in LDL of d 1.050-1.100 g/ml, in which the radioactive profile shifted towards lighter particles of the d 1.024-1.050 g/ml species; this shift was partially dependent on the LDL receptor, since it was more pronounced in the methylated subfraction. Furthermore, a net increase in the radioactive content of gradient subfractions 7 to 9 (d 1.032-1.042 g/ml) was found 10 hr after injection of methylated LDL of d 1.050-1.100 g/ml, at which time the bulk of LDL radioactivity had been removed from plasma. Several mechanisms, acting alone or in combination, may account for these findings; among them, some degree of transformation of dense to lighter LDL species appears a prerequisite. In conclusion, our data attest to the structural heterogeneity of circulating LDL in the guinea pig, and suggest that the intravascular processing and metabolism of LDL particle subspecies is directly related to their structure and physicochemical properties.

摘要

在豚鼠体内对低密度脂蛋白(LDL,密度1.024 - 1.100 g/ml)的结构和代谢异质性进行了研究。通过连续超速离心分离出两个LDL亚组分,密度分别为1.024 - 1.050 g/ml和1.050 - 1.100 g/ml;二者都富含胆固醇酯和载脂蛋白B - 100,前者具有异质性,呈现三种粒径的颗粒,直径分别为26.9、25.6和24.7 nm,而密度较大的亚组分相对均一,包含单一的较小颗粒(直径23.6 nm)。在豚鼠体内,这两个LDL亚组分的分数分解代谢率(FCR)相似(约0.090池/小时)。对每个亚组分进行还原甲基化修饰后,FCR同样降低,表明70 - 80%的降解通过细胞LDL受体途径发生。然而,根据放射性标记的天然或化学修饰LDL注射后不同时间密度梯度组分的放射性含量所确定的这些LDL亚组分的血管内代谢情况,往往有所不同。因此,虽然较轻亚组分中放射性标记的载脂蛋白B - 100在长达48小时内保持初始密度分布,但甲基化对应物的放射性分布发生了变化,较轻密度梯度组分(密度1.027 - 1.032 g/ml)中的放射性比例增加,而较密度组分(密度1.037 - 1.042 g/ml)中的放射性比例降低。密度为1.050 - 1.100 g/ml的LDL发生了更显著的转变,其放射性分布向密度为1.024 - 1.050 g/ml的较轻颗粒转移;这种转移部分依赖于LDL受体,因为在甲基化亚组分中更为明显。此外,注射密度为1.050 - 1.100 g/ml的甲基化LDL 10小时后,发现梯度亚组分7至9(密度1.032 - 1.042 g/ml)的放射性含量净增加,此时大部分LDL放射性已从血浆中清除。单独或共同起作用的几种机制可能解释这些发现;其中,一定程度的从致密LDL颗粒向较轻LDL颗粒的转变似乎是一个前提条件。总之,我们的数据证明了豚鼠体内循环LDL的结构异质性,并表明LDL颗粒亚类的血管内加工和代谢与其结构和物理化学性质直接相关。

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