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新生仔猪小肠细胞系(IPEC-1)脂蛋白和载脂蛋白的分泌

Lipoprotein and apolipoprotein secretion by a newborn piglet intestinal cell line (IPEC-1).

作者信息

Gonzalez-Vallina R, Wang H, Zhan R, Berschneider H M, Lee R M, Davidson N O, Black D D

机构信息

Department of Pediatrics, Arkansas Children's Hospital, University of Arkansas for Medical Sciences, Little Rock 72202, USA.

出版信息

Am J Physiol. 1996 Aug;271(2 Pt 1):G249-59. doi: 10.1152/ajpgi.1996.271.2.G249.

Abstract

The aim of these studies was to characterize the synthesis and secretion of lipoproteins and apolipoprotein B (apo B) and apo A-I by a newborn swine intestinal epithelial cell line (IPEC-1). Differentiated cells exhibited enterocytic features, including microvilli. [3H] oleic acid was taken up and incorporated into cellular lipids and secreted into the basolateral medium in lipoproteins. Total apo B and apo A-I secreted increased with oleic acid incubation. However, cellular apo B and apo A-I content did not change. Whereas undifferentiated cells synthesized and secreted only apo B-100, both apo B-100 and apo B-48 were produced by differentiated cells. The ratio of radiolabeled apo B-48 to apo B-100 in both basolateral medium and cell homogenate increased with oleic acid treatment after 24-h steady-state labeling. However, apo B mRNA editing was unchanged, indicating posttranslational regulation of this ratio. Pulse-chase radiolabeling demonstrated no major changes in cellular or basolateral medium apolipoprotein labeling kinetics with oleic acid or dexamethasone incubation. The dissociation of apo B and apo A-I mass secretion from the secretion of radiolabeled apo B and apo A-I in response to oleic acid absorption suggests the presence of an intracellular pool of apolipoprotein with a slow turnover that is mobilized for secretion in response to fatty acid uptake.

摘要

这些研究的目的是对新生猪肠道上皮细胞系(IPEC-1)脂蛋白、载脂蛋白B(apo B)和载脂蛋白A-I(apo A-I)的合成与分泌进行表征。分化细胞呈现出肠细胞特征,包括微绒毛。[3H]油酸被摄取并掺入细胞脂质中,然后以脂蛋白的形式分泌到基底外侧培养基中。随着油酸孵育,分泌的总apo B和apo A-I增加。然而,细胞内apo B和apo A-I的含量没有变化。未分化细胞仅合成和分泌apo B-100,而分化细胞则产生apo B-100和apo B-48。在24小时稳态标记后,基底外侧培养基和细胞匀浆中放射性标记的apo B-48与apo B-100的比率随油酸处理而增加。然而,apo B mRNA编辑没有变化,表明该比率存在翻译后调控。脉冲追踪放射性标记显示,油酸或地塞米松孵育后,细胞内或基底外侧培养基中载脂蛋白的标记动力学没有重大变化。响应油酸吸收,apo B和apo A-I的质量分泌与放射性标记的apo B和apo A-I的分泌解离,表明存在一个周转缓慢的细胞内载脂蛋白池,该池在响应脂肪酸摄取时被动员用于分泌。

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