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在没有胞质溶胶的情况下膜锚定转化生长因子α的激活释放。

Activated release of membrane-anchored TGF-alpha in the absence of cytosol.

作者信息

Bosenberg M W, Pandiella A, Massagué J

机构信息

Cell Biology and Genetics Program, Memorial Sloan-Kettering Cancer Center, New York 10021.

出版信息

J Cell Biol. 1993 Jul;122(1):95-101. doi: 10.1083/jcb.122.1.95.

Abstract

The ectodomain of proTGF-alpha, a membrane-anchored growth factor, is converted into soluble TGF-alpha by a regulated cellular proteolytic system that recognizes proTGF-alpha via the C-terminal valine of its cytoplasmic tail. In order to define the biochemical components involved in proTGF-alpha cleavage, we have used cells permeabilized with streptolysin O (SLO) that have been extensively washed to remove cytosol. PMA, acting through a Ca(2+)-independent protein kinase C, activates cleavage as efficiently in permeabilized cells as it does in intact cells. ProTGF-alpha cleavage is also stimulated by GTP gamma S through a mechanism whose pharmacological properties suggest the involvement of a heterotrimeric G protein acting upstream of the PMA-sensitive Ca(2+)-independent protein kinase C. Activated proTGF-alpha cleavage is dependent on ATP hydrolysis, appears not to require vesicular traffic, and acts specifically on proTGF-alpha that has reached the cell surface. These results indicate that proTGF-alpha is cleaved from the cell surface by a regulated system whose signaling, recognition, and proteolytic components are retained in cells devoid of cytosol.

摘要

前转化生长因子α(proTGF-α)是一种膜锚定生长因子,其胞外结构域通过一种受调控的细胞蛋白水解系统转化为可溶性转化生长因子α(TGF-α),该系统通过其胞质尾的C末端缬氨酸识别proTGF-α。为了确定参与proTGF-α切割的生化成分,我们使用了经链球菌溶血素O(SLO)通透处理的细胞,这些细胞经过广泛洗涤以去除胞质溶胶。佛波酯(PMA)通过一种不依赖Ca²⁺的蛋白激酶C起作用,在通透细胞中激活切割的效率与在完整细胞中相同。GTPγS也通过一种机制刺激proTGF-α的切割,其药理学特性表明一种异源三聚体G蛋白参与其中,该蛋白作用于对PMA敏感的不依赖Ca²⁺的蛋白激酶C的上游。激活的proTGF-α切割依赖于ATP水解,似乎不需要囊泡运输,并且特异性作用于已到达细胞表面的proTGF-α。这些结果表明,proTGF-α在细胞表面被一个受调控的系统切割,该系统的信号传导、识别和蛋白水解成分保留在没有胞质溶胶的细胞中。

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