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蛋白转化酶 PC7 从质膜内化是由一个新的基序介导的。

Internalization of proprotein convertase PC7 from plasma membrane is mediated by a novel motif.

机构信息

Department of Human Genetics, University of Leuven, Leuven, Belgium.

出版信息

J Biol Chem. 2012 Mar 16;287(12):9052-60. doi: 10.1074/jbc.M111.306407. Epub 2012 Jan 30.

Abstract

Proprotein convertase 7 (PC7) is a member of the subtilisin-like proprotein convertase family, which is involved in the endoproteolysis of a variety of precursor proteins. Under steady state conditions, PC7 is mainly localized in the trans-Golgi network, but a small fraction is found at the cell surface. So far, no sorting signals for membrane trafficking have been identified in PC7. In this study, we have examined the internalization of PC7 from the plasma membrane. Our results show that internalization of PC7 is mediated by clathrin-coated vesicles. After inhibition of clathrin-mediated endocytosis using hypertonic conditions or the small molecule inhibitor, Pitstop 2, PC7 accumulated at the plasma membrane. Furthermore, PC7 was present in isolated clathrin-coated vesicles. To determine the internalization motif, constructs were generated in which parts of the N and C terminus of the cytoplasmic tail of PC7 were deleted, and chimeric proteins were constructed consisting of the luminal and transmembrane domains of Tac (CD25) and parts of the cytoplasmic domain of PC7. Antibody uptake experiments as well as surface biotinylation experiments demonstrated that the region between Ala(713) and Cys(726) in the cytoplasmic domain of PC7 is essential and sufficient for the internalization of PC7 but not for trans-Golgi network localization. Individual amino acids in this region were substituted with alanine, which identified Pro, Leu, and Cys as the essential amino acids. In conclusion, internalization of PC7 depends on a short transferable sequence in the cytoplasmic tail, which contains the three crucial amino acids PLC.

摘要

脯氨酸内切酶 7(PC7)是枯草杆菌蛋白酶样蛋白前体转化酶家族的一员,参与多种前体蛋白的内切蛋白酶解。在稳态条件下,PC7 主要定位于反式高尔基体网络,但一小部分位于细胞表面。到目前为止,PC7 中尚未发现用于膜运输的分选信号。在这项研究中,我们研究了 PC7 从质膜内化的过程。结果表明,PC7 的内化是由网格蛋白包被小泡介导的。用高渗条件或小分子抑制剂 Pitstop 2 抑制网格蛋白介导的内吞作用后,PC7 积累在质膜上。此外,PC7 存在于分离的网格蛋白包被小泡中。为了确定内化基序,构建了缺失 PC7 胞质尾部的 N 端和 C 端部分的构建体,并构建了由 Tac(CD25)的腔和跨膜结构域以及 PC7 的胞质结构域的部分组成的嵌合蛋白。抗体摄取实验和表面生物素化实验表明,PC7 胞质尾部的 Ala(713)和 Cys(726)之间的区域对于 PC7 的内化是必需和充分的,但对于反式高尔基体网络定位则不是必需的。该区域的单个氨基酸被替换为丙氨酸,确定 PLC 中的 Pro、Leu 和 Cys 是必需氨基酸。总之,PC7 的内化依赖于胞质尾部的一个短的可转移序列,该序列包含三个关键氨基酸 PLC。

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