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从培养的人脐静脉内皮细胞中分离出的血管性血友病因子储存细胞器(魏-帕小体)的组成。

Composition of the von Willebrand factor storage organelle (Weibel-Palade body) isolated from cultured human umbilical vein endothelial cells.

作者信息

Ewenstein B M, Warhol M J, Handin R I, Pober J S

出版信息

J Cell Biol. 1987 May;104(5):1423-33. doi: 10.1083/jcb.104.5.1423.

Abstract

von Willebrand factor (VWF) is a large, adhesive glycoprotein that is biosynthesized and secreted by cultured endothelial cells (EC). Although these cells constitutively release VWF, they also contain a storage pool of this protein that can be rapidly mobilized. In this study, a dense organelle fraction was isolated from cultured umbilical vein endothelial cells by centrifugation on a self-generated Percoll gradient. Stimulation of EC by 4-phorbol 12-myristate 13-acetate (PMA) resulted in the disappearance of this organelle fraction and the synchronous loss of Weibel-Palade bodies as judged by immunoelectron microscopy. Electrophoretic and serologic analyses of biosynthetically labeled dense organelle fraction revealed that it is comprised almost exclusively of VWF and its cleaved pro sequence. These two polypeptides were similarly localized exclusively to Weibel-Palade bodies by ultrastructural immunocytochemistry. The identity of the dense organelle as the Weibel-Palade body was further established by direct morphological examination of the dense organelle fraction. The VWF derived from this organelle is distributed among unusually high molecular weight multimers composed of fully processed monomeric subunits and is rapidly and quantitatively secreted in unmodified form after PMA stimulation. These studies: establish that the Weibel-Palade body is the endothelial-specific storage organelle for regulated VWF secretion; demonstrate that in cultured EC, the VWF concentrated in secretory organelles is of unusually high molecular weight and that this material may be rapidly mobilized in unmodified form; imply that proteolytic processing of VWF involved in regulated secretion takes place after translocation to the secretory organelle; provide a basis for further studies of intracellular protein trafficking in EC.

摘要

血管性血友病因子(VWF)是一种由培养的内皮细胞(EC)生物合成并分泌的大型黏附糖蛋白。尽管这些细胞持续释放VWF,但它们也含有该蛋白的储存池,可被快速调动。在本研究中,通过在自生成的Percoll梯度上离心,从培养的脐静脉内皮细胞中分离出一个致密细胞器组分。用4-佛波醇12-肉豆蔻酸酯13-乙酸酯(PMA)刺激内皮细胞,通过免疫电子显微镜判断,导致该细胞器组分消失以及Weibel-Palade小体同步丢失。对生物合成标记的致密细胞器组分进行电泳和血清学分析表明,它几乎完全由VWF及其裂解的前体序列组成。通过超微结构免疫细胞化学,这两种多肽同样仅定位于Weibel-Palade小体。通过对致密细胞器组分的直接形态学检查,进一步确定了致密细胞器为Weibel-Palade小体。源自该细胞器的VWF分布在由完全加工的单体亚基组成的异常高分子量多聚体中,并在PMA刺激后以未修饰的形式快速定量分泌。这些研究:确定Weibel-Palade小体是内皮细胞特异性储存细胞器,用于调节VWF分泌;证明在培养的内皮细胞中,集中在分泌细胞器中的VWF具有异常高分子量,且该物质可能以未修饰的形式快速调动;暗示参与调节性分泌的VWF的蛋白水解加工发生在转运至分泌细胞器之后;为进一步研究内皮细胞中的细胞内蛋白质运输提供了基础。

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