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激素原转化酶3与膜脂筏的关联。

Association of prohormone convertase 3 with membrane lipid rafts.

作者信息

Blázquez M, Docherty K, Shennan K I

机构信息

Department of Molecular and Cell Biology, Institute of Medical Sciences, University of Aberdeen, Foresterhill, Aberdeen AB25 2ZD, UK.

出版信息

J Mol Endocrinol. 2001 Aug;27(1):107-16. doi: 10.1677/jme.0.0270107.

DOI:10.1677/jme.0.0270107
PMID:11463581
Abstract

Prohormone convertase 3 (PC3) is a neuroendocrine-specific member of the subtilisin-kexin family, involved in the intracellular processing and maturation of prohormones and proneuropeptides. PC3 is synthesised as a proprotein that undergoes two different cleavages resulting in the mature PC3 and the enzymatically active PC3DeltaC. In vitro translated proPC3 and proPC3DeltaC bind to trans-Golgi network (TGN)/granule-enriched membranes from the AtT20 neuroendocrine cell line in a pH-dependent manner suggesting both a dominant role for the pro-region in membrane association and that the C-terminal region is not essential. However, while PC3 bound to membranes the majority of PC3DeltaC did not, suggesting that either the pro-region or the C-terminal region of PC3 is required for membrane association. Removal of peripheral membrane proteins did not affect the binding properties of any of the in vitro translated proteins. Chromaffin granule membranes (CGMs) were used to study the binding characteristics of endogenous PC3 and its active C-terminal truncated counterpart (PC3DeltaC). Incubation of CGMs with Triton X-100 did not completely solubilise either of these forms of PC3. Moreover, both PC3 and PC3DeltaC remained associated with detergent-resistant membrane microdomains, termed lipid rafts, purified from CGMs. The data raise the possibility that PC3 and PC3DeltaC are sorted to the regulated secretory pathway via their association with membrane lipid rafts.

摘要

激素原转化酶3(PC3)是枯草杆菌蛋白酶-凯新家族中神经内分泌特异性成员,参与激素原和前神经肽的细胞内加工与成熟。PC3最初作为一种前体蛋白合成,经过两次不同的切割,产生成熟的PC3和具有酶活性的PC3DeltaC。体外翻译的前体PC3和前体PC3DeltaC以pH依赖的方式与AtT20神经内分泌细胞系的反式高尔基体网络(TGN)/富含颗粒的膜结合,这表明前体区域在膜结合中起主导作用,且C末端区域并非必需。然而,虽然PC3与膜结合,但大多数PC3DeltaC却不与膜结合,这表明PC3的前体区域或C末端区域对于膜结合是必需的。去除外周膜蛋白并不影响任何一种体外翻译蛋白的结合特性。嗜铬粒细胞膜(CGM)用于研究内源性PC3及其活性C末端截短对应物(PC3DeltaC)的结合特性。用Triton X-100孵育CGM并不能完全溶解这两种形式的PC3。此外,PC3和PC3DeltaC都与从CGM中纯化的抗去污剂膜微结构域(即脂筏)保持结合。这些数据增加了一种可能性,即PC3和PC3DeltaC通过与膜脂筏的结合被分选到调节性分泌途径。

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Arch Histol Cytol. 1996 Aug;59(3):261-71. doi: 10.1679/aohc.59.261.

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