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鸡肝高密度脂蛋白的生物合成:新生细胞内高密度脂蛋白的性质

Biosynthesis of high density lipoprotein by chicken liver: nature of nascent intracellular high density lipoprotein.

作者信息

Banerjee D, Redman C M

出版信息

J Cell Biol. 1983 Mar;96(3):651-60. doi: 10.1083/jcb.96.3.651.

Abstract

Young chickens were administered L-[(3)H]leucine and after 10 or 30 min the livers were removed and fractioned into rough (RER) and smooth (SER) endoplasmic reticulum fractions and into light, intermediate, and heavy golgo cell fractions. The labeled high density lipoprotein (HDL), contained within these intracellular organelles was isolated either by immunoprecipitation using rabbit antiserum to rooster HDL, or by ultracentrifugal glotation between densities 1.063 and 1.21 g/ml. The radioactive apoproteins of nascent HDL were analyzed by SDS PAGE and detected by fluorography. Analyses of radioactive apoproteins obtained by immunoprecipitation from the contents of the RER, the SER, and the three golgi complex fractions revealed only one apoprotein, A1. The C peptide present in serum HDL was not detected intracellularly. The radioactive apoprotein A1 which is present within the cisternae of the RER and the SER fractions failed to float, whereas apoprotein A1, present within the golgi apparatus, readily floated between densities 1.063 and 1.21 g/ml. The HDL particles, isolated by flotation from the golgi apparatus content, were further characterized by lipid and protein analyses and by electron microscopy. Golgi HDL particles have the same density as serum HDL. On a percentage basis, golgi HDL contains less protein and more phospholipids than does serum HDL. Morphologically, golgi HDL is different in appearance from serum HDL. It is more heterogeneous in size, with most of the particles ranging 8.3-25 nm in diameter. The spherical particles contain small membrane tails. Occasionally, a few disk-shaped bilayer structures are also found within the golgi apparatus. These studies show that the newly synthesized apoprotein A1, present within the RER and the SER cell fractions, is not fully complexed with lipid and that apoprotein A1 does not acquire sufficient lipid to float at the proper HDL density until it enters the golgi apparatus. The difference in chemical composition and the heterogeneous size of golgi HDL may be attributed to the different stages of HDL maturation.

摘要

给幼鸡注射L-[(3)H]亮氨酸,10或30分钟后取出肝脏,将其分离成粗面内质网(RER)和滑面内质网(SER)组分,以及轻、中、重高尔基体细胞组分。这些细胞内细胞器中所含的标记高密度脂蛋白(HDL),可通过用兔抗公鸡HDL血清进行免疫沉淀,或通过在密度1.063至1.21 g/ml之间进行超速离心浮选来分离。通过SDS-PAGE分析新生HDL的放射性载脂蛋白,并通过荧光自显影进行检测。对通过免疫沉淀从RER、SER和三个高尔基体组分的内容物中获得的放射性载脂蛋白进行分析,仅发现一种载脂蛋白A1。血清HDL中存在的C肽在细胞内未被检测到。存在于RER和SER组分池中的放射性载脂蛋白A1未能漂浮,而存在于高尔基体中的载脂蛋白A1则很容易在密度1.063至1.21 g/ml之间漂浮。通过从高尔基体内容物中浮选分离得到的HDL颗粒,通过脂质和蛋白质分析以及电子显微镜进一步表征。高尔基体HDL颗粒与血清HDL具有相同的密度。按百分比计算,高尔基体HDL所含蛋白质比血清HDL少,磷脂比血清HDL多。从形态学上看,高尔基体HDL的外观与血清HDL不同。其大小更具异质性,大多数颗粒直径在8.3至25 nm之间。球形颗粒含有小的膜尾。偶尔,在高尔基体中也会发现一些盘状双层结构。这些研究表明,存在于RER和SER细胞组分中的新合成载脂蛋白A1并未与脂质完全复合,并且载脂蛋白A1在进入高尔基体之前不会获得足够的脂质以在适当的HDL密度下漂浮。高尔基体HDL在化学组成和大小异质性方面的差异可能归因于HDL成熟的不同阶段。

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