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负鼠肾细胞培养中白蛋白的受体介导内吞作用:近端肾小管蛋白重吸收的模型

Receptor-mediated endocytosis of albumin in cultured opossum kidney cells: a model for proximal tubular protein reabsorption.

作者信息

Schwegler J S, Heppelmann B, Mildenberger S, Silbernagl S

机构信息

Physiologisches Institut, Universität Würzburg, Federal Republic of Germany.

出版信息

Pflugers Arch. 1991 May;418(4):383-92. doi: 10.1007/BF00550876.

Abstract

The accumulation of fluorescein (FITC)-labelled bovine albumin was measured against the extracellular-fluid-phase marker FITC-inulin within confluent monolayers of the opossum kidney cell line OK. Fluorescence and electron microscopic pictures show that FITC-albumin is taken up by endocytosis and appears in a vesicular intracellular distribution. The uptake of FITC-albumin was quantified by measuring the cell-adherent fluorescence fluorimetrically. FITC-albumin uptake shows a time- and concentration-dependent saturation kinetics in contrast to the non-saturable FITC-inulin uptake, and exceeds the latter more than tenfold at low concentrations. Half-maximum saturation occurs at 20-30 mg/l. Initial FITC-albumin uptake/mg protein is stimulated by cell maturation, being six-to sevenfold higher in the confluent than in the subconfluent state, while FITC-inulin uptake is unchanged. Both an elevation of ambient osmolality to 600-750 mOsm/kg and disruption of the cytoskeleton by cytochalasin B (0.1 mmol/l) reduce initial FITC-albumin uptake by 50%-60% in a non-additive fashion. Albumin endocytosis is reduced both in acidic (pH 5.4) and alkaline (pH 8.4) medium, but does not depend on extracellular sodium, calcium or chloride. High concentrations of fetal calf serum or unlabelled albumin reduce FITC-albumin endocytosis dose-dependently. The present study is the first to investigate both the protein uptake and the fluid-phase endocytosis in a cultured proximal tubular cell line, using these cells as a model system-for proximal tubular protein reabsorption.

摘要

在负鼠肾细胞系OK的汇合单层细胞中,以细胞外液相标记物异硫氰酸荧光素(FITC)-菊粉为对照,测定了异硫氰酸荧光素(FITC)标记的牛血清白蛋白的蓄积情况。荧光和电子显微镜照片显示,FITC-白蛋白通过内吞作用被摄取,并以囊泡状的细胞内分布形式出现。通过荧光法测量细胞附着荧光来定量FITC-白蛋白的摄取。与非饱和的FITC-菊粉摄取不同,FITC-白蛋白摄取呈现出时间和浓度依赖性的饱和动力学,并且在低浓度时比后者高出十倍以上。半数最大饱和度出现在20 - 30mg/l。细胞成熟会刺激初始FITC-白蛋白摄取/毫克蛋白,汇合状态下比亚汇合状态高6至7倍,而FITC-菊粉摄取不变。将环境渗透压提高到600 - 750mOsm/kg以及用细胞松弛素B(0.1mmol/l)破坏细胞骨架,均以非累加方式使初始FITC-白蛋白摄取减少50% - 60%。白蛋白内吞作用在酸性(pH 5.4)和碱性(pH 8.4)培养基中均减少,但不依赖于细胞外的钠、钙或氯。高浓度的胎牛血清或未标记的白蛋白会剂量依赖性地减少FITC-白蛋白内吞作用。本研究首次使用这些细胞作为近端肾小管蛋白重吸收的模型系统,研究了培养的近端肾小管细胞系中的蛋白摄取和液相内吞作用。

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